Diagnosis of melanoma by nucleic acid analysis

ABSTRACT

The present invention provides methods for diagnosing melanoma in a subject by analyzing nucleic acid molecules obtained from the subject. The present invention also provides methods for distinguishing melanoma from dysplastic nevi and/or normal pigmented skin. The methods include analyzing expression or mutations in epidermal samples, of one or more skin markers. The methods can include the use of a microarray to analyze gene or protein profiles from a sample.

CROSS REFERENCE TO RELATED APPLICATION(S)

This application claims the benefit of priority under 35 U.S.C. § 119(e) of U.S. Ser. No. 60/927,802, filed May 4, 2007, of U.S. Ser. No. 60/928,248, filed May 7, 2007, of U.S. Ser. No. 60/984,326, filed Oct. 31, 2007, of U.S. Ser. No. 60/984,684, filed Nov. 1, 2007, and of U.S. Ser. No. 61/018,850, filed Jan. 3, 2008, the entire content of each is incorporated herein by reference.

BACKGROUND OF THE INVENTION

1. Field of the Invention

The invention relates generally to methods of characterizing pigmented skin lesions suspected of being melanomas using primarily non-invasive skin sampling.

2. Background Information

Melanoma is a serious form of skin cancer in humans. It arises from the pigment cells (melanocytes), usually in the skin. The incidence of melanoma is increasing at the fastest rate of all cancers in the United States with a lifetime risk of 1 in 68. Although melanoma accounts for only 4% of all dermatologic cancers, it is responsible for 80% of all deaths from skin cancers. It has long been realized that recognition and diagnosis of melanoma, when it is early stage disease, is key to its cure.

Given this, it is imperative that research be carried out not only on therapeutics for melanoma, but also on all aspects of melanoma including prevention and detection. Most of these deaths from melanoma could have been prevented if the melanomas, initially located on the skin, could have been detected in their early stages. The ability to cure melanoma in its earliest skin stage, in situ, is virtually 100% if the melanoma is adequately surgically excised. If the melanoma is caught in a later stage, where it has invaded to a depth of 4 mm or more, the ten-year survival rate is less than 50%. If the melanoma is not detected until it has spread to distant parts of the body (Stage 1V), the prognosis is dismal, with only 7-9% of patients surviving 5 years, with the median survival time being 8-9 months. The long-term “cure” rate for Stage 1V melanoma is only 1-2%.

To advance early detection of melanoma, several things must be improved. People need to be better educated with regards to the risks of melanoma and how to prevent and detect it on their own skin. Also physicians need to be more alert to the possibility of melanoma and be better trained in detection. But even if these two areas are improved, the diagnosis of melanoma on the skin is still difficult. Studies have shown that even expert clinicians working in pigmented lesion clinics where melanoma is their specialty are only able to determine whether a suspicious pigmented lesion is melanoma or not with 60-80% sensitivity. This leads to the need for surgical biopsy of large numbers of pigmented lesions for every melanoma that is detected, and, doubtless, to the missing of some melanomas in their early stages.

In current practice melanoma is diagnosed by biopsy and histopathological examination; approximately 20 to 30 biopsies must be performed to find one melanoma and even then some melanomas are missed in the earliest stage. The limitations of visual detection are apparent to dermatologists who are constantly searching for ways to better determine whether suspicious lesions are melanoma or not without having to cut them out first. To this end, epiluminescence microscopy (ELM) has come into use. This is a method whereby lesions are looked at using a device that simultaneously magnifies the lesion while reducing visual interference from refractive index differences at the skin-air interface. While ELM does give a different view, it is of limited improvement. Studies have shown that until one becomes fairly skilled in utilizing the instrument, sensitivity in detection of melanoma actually decreases. Even very skilled users of ELM improve their ability to detect melanomas only by 5-10%. This still leads to an unacceptable sensitivity in detection and the need to biopsy large numbers of benign lesions to detect a few melanomas. And again, some melanomas will be missed completely in their early stages.

Clearly there is a need for further development of technology that will enable physicians to determine the nature and extent of suspicious lesions of the skin. Such technology would ideally directly assay the physiology of the suspect lesion to enable a sensitive diagnosis.

SUMMARY OF THE INVENTION

The present invention is based, in part, on the discovery that analysis of nucleic acid molecules or of protein expression products of nucleic acid molecules from specific genes can be used to characterize skin lesions in a subject. The method provides valuable genetic information based on DNA, messenger RNA, or protein expression products obtained therefrom, for example.

In one embodiment, the method involves use of a non-invasive approach for recovering nucleic acids such as DNA or messenger RNA or proteins from the surface of skin via a tape stripping procedure that permits a direct quantitative and qualitative assessment of biomarkers. Although tape-harvested nucleic acid and protein expression products are shown to be comparable in quality and utility to recovering such molecules by biopsy, the non-invasive method provides information regarding cells of the outermost layers of the skin that may not be obtained using biopsy samples. Finally, the non-invasive method is far less traumatic than a biopsy.

Thus, the non-invasive method is used to capture cells on pigmented skin lesions that are suspected of being early melanomas. Nucleic acid molecules obtained from skin cells captured by the non-invasive method are analyzed in order to diagnose the nature of the lesion (e.g., malignant melanoma). In one embodiment, a nucleic acid molecule is amplified prior to analysis. Secondary outcomes could include tests for diagnosis and prognosis of a variety of pigmented skin lesions and even to predict a therapeutic regimen. In another embodiment, the skin cells are lysed to extract one or more proteins, which are then quantitated to diagnose the nature of the lesion. It should be understood that the methods of the invention are not limited to non-invasive techniques for obtaining skin samples. For example, but not by limitation, one of skill in the art would know other techniques for obtaining a skin sample such as scraping of the skin, biopsy, suction, blowing and other techniques. As described herein, non-invasive tape stripping is an illustrative example for obtaining a skin sample.

In another embodiment, the methods involve detection of one or more mutations in the nucleic acid sequence of the nucleic acid molecule obtained from the skin. Such mutations may be a substitution, a deletion, and/or an insertion of the nucleic acid sequence that results in a diseased state in the subject from which the skin sample is obtained.

In one embodiment, the nucleic acid molecule analyzed is listed in Tables 1-6. For example, in one embodiment, the gene analyzed is any one or more of human mRNA for tyrosinase-related protein 1, LIM homeobox 2, melan-A, spermidine/spermine N1-acetyltransferase, NDRG family member 2, carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2, syndecan binding protein (syntenin), crystallin, alpha B, endothelin receptor type B, tetratricopeptide repeat domain 3, WAP four-disulfide core domain 3, cytochrome P450 (family 1, subfamily B, polypeptide 1), p8 protein (candidate of metastasis 1), interferon gamma-inducible protein 16, dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2), solute carrier family 39 (zinc transporter), member 6, heat shock 70 kDa protein 2, vesicle-associated membrane protein 2 (synaptobrevin 2), Similar to AI661453 protein, and transient receptor potential cation channel (subfamily M, member 1), tyrosinase (oculocutaneous albinism IA), endothelin receptor type B, tetratricopeptide repeat domain 3, syndecan binding protein (syntenin), v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog, OTU domain, ubiquitin aldehyde binding 1, protein phosphatase 1 regulatory (inhibitor) subunit 12A, calponin 2, dishevelled dsh homolog 3 (Drosophila), tribbles homolog 2 (Drosophila), mucolipin 3, actinin alpha 4, ribosomal protein S15, CDC37 cell division cycle 37 homolog (S. cerevisiae), jumonji domain containing 3, v-maf musculoaponeurotic fibrosarcoma oncogene homolog B (avian), c-Maf-inducing protein, myosin heavy polypeptide 14, Hypothetical protein MGC40222, or combinations thereof. In one embodiment, the nucleic acid molecule is from one or more genes listed in Table 6.

Accordingly, provided herein is a method for characterizing and/or diagnosing melanoma in a subject, including obtaining a nucleic acid molecule or protein by biopsy of a skin lesion on the subject, and analyzing the nucleic acid molecule to distinguish melanoma from dysplastic nevi and/or normal pigmented skin in the subject. In this method, at least one nucleic acid molecule whose expression is informative of melanoma is detected in the epidermal sample. In one example, expression of one or more of the genes listed in Tables 1-6, or a combination thereof, is detected in the epidermal sample to characterize the melanoma. In one embodiment, the nucleic acid molecule is from one or more genes listed in any of Tables 1-6, or any combination thereof. In another embodiment, the gene is any one or more of human mRNA for tyrosinase-related protein 1, LIM homeobox 2, melan-A, spermidine/spermine N1-acetyltransferase, NDRG family member 2, carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2, syndecan binding protein (syntenin), crystallin, alpha B, endothelin receptor type B, tetratricopeptide repeat domain 3, WAP four-disulfide core domain 3, cytochrome P450 (family 1, subfamily B, polypeptide 1), p8 protein (candidate of metastasis 1), interferon gamma-inducible protein 16, dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2), solute carrier family 39 (zinc transporter), member 6, heat shock 70 kDa protein 2, vesicle-associated membrane protein 2 (synaptobrevin 2), Similar to AI661453 protein, and transient receptor potential cation channel (subfamily M, member 1), tyrosinase (oculocutaneous albinism IA), endothelin receptor type B, tetratricopeptide repeat domain 3, syndecan binding protein (syntenin), v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog, OTU domain, ubiquitin aldehyde binding 1, protein phosphatase 1 regulatory (inhibitor) subunit 12A, calponin 2, dishevelled dsh homolog 3 (Drosophila), tribbles homolog 2 (Drosophila), mucolipin 3, actinin alpha 4, ribosomal protein S15, CDC37 cell division cycle 37 homolog (S. cerevisiae), jumonji domain containing 3, v-maf musculoaponeurotic fibrosarcoma oncogene homolog B (avian), c-Maf-inducing protein, myosin heavy polypeptide 14, Hypothetical protein MGC40222, or combinations thereof. In one embodiment, the nucleic acid molecule is from one or more genes listed in Table 6.

The non-invasive methods of the invention involve applying an adhesive tape to a target area of skin in a manner sufficient to isolate a sample adhering to the adhesive tape, wherein the sample includes nucleic acid molecules or proteins. Typically, at least one nucleic acid molecule or protein whose expression is informative of melanoma is detected in the sample. The method of characterizing skin using tape stripping has a number of applications, such as the following: (i) disease classification/subclassification; (ii) monitoring disease severity and progression; (iii) monitoring treatment efficacy; and (iv) prediction of a particular treatment regimen. All of these applications, which themselves represent embodiments disclosed herein, preferably use non-invasive sampling to recover information that is otherwise difficult or impractical to recover (e.g., through the use of biopsies). The information may be contained in the DNA, protein, or RNA of skin cells close to the surface of the skin. In one example, expression of one or more of the genes listed in Tables 1-6, or a combination thereof, is detected in the sample to characterize the sample. This exemplary method is particularly useful for distinguishing melanoma from dysplastic nevi and/or normal pigmented skin. In one embodiment, expression of one or more of the genes listed in Table 6 is detected in the sample to characterize the sample.

As such, also provided herein is a method for distinguishing melanoma from dysplastic nevi and/or normal pigmented skin in a subject, including applying an adhesive tape to a target area of skin in a manner sufficient to isolate a sample adhering to the adhesive tape, wherein the sample includes nucleic acid molecules. At least one nucleic acid molecule whose expression is informative of melanoma is detected in the sample. In one example, expression of one or more of the genes listed in Tables 1-6, or a combination thereof, is detected in the sample to characterize the melanoma. In one embodiment, expression of one or more of the genes listed in Table 6 is detected in the sample to characterize the melanoma.

Other embodiments are based in part on the discovery that for tape stripping of the skin, non-polar, pliable, adhesive tapes, especially pliable tapes with rubber adhesive, are more effective than other types of adhesive tapes. Using pliable tapes with rubber adhesives, as few as 10 or less tape strippings and in certain examples as few as 4 or even 1 tape stripping can be used to isolate and/or detect nucleic acid molecules from the epidermal layer of the skin.

In another embodiment, the methods of the invention provide for characterization of a skin lesion in situ, including application of a detectably labeled probe directly to a skin lesion for visual analysis. At least one nucleic acid molecule whose expression is informative of melanoma or dysplastic nevi or normal skin is detected on the skin lesion or surrounding margin or tissue using a specific probe. In one example, expression of one or more of the genes listed in Tables 1-6, or a combination thereof, is detected on the skin lesion or surrounding margin or tissue to characterize the melanoma. In one embodiment, expression of one or more of the genes listed in Table 6 is detected in the sample to characterize the melanoma.

Also provided herein is a method for diagnosing a disease state by establishing a gene expression pattern of a target area suspected of being melanoma on the skin of a subject and comparing the subject's gene expression profile to a reference gene expression profile obtained from a corresponding normal skin sample. In one embodiment, the target area of the skin simultaneously expresses a plurality of genes at the protein level that are markers for melanoma. In another embodiment, the genes are listed in Tables 1-6. In another embodiment, the genes are listed in Table 6.

In one embodiment, the method of diagnosing a disease state involves detection of one or more mutations in the nucleic acid sequence of the gene. Such mutations may be a substitution, a deletion, and/or an insertion of the nucleic acid sequence that results in a diseased state in the subject from which the skin sample is obtained. In one embodiment, the genes are listed in Tables 1-6. In another embodiment, the genes are listed in Table 6.

In another aspect, the invention provides kits for characterizing a skin lesion in a subject. In one embodiment, the kit includes a skin sample collection device, such as a biopsy needle or an adhesive tape for non-invasive tape stripping, and one or more probes or primers that selectively bind to one or more nucleic acid molecules in any of Tables 1-6, or to a nucleic acid or protein expression product of a nucleic acid molecule in any of Tables 1-6. For example, in one embodiment, the gene analyzed is any one or more of human mRNA for tyrosinase-related protein 1, LIM homeobox 2, melan-A, spermidine/spermine N1-acetyltransferase, NDRG family member 2, carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2, syndecan binding protein (syntenin), crystallin, alpha B, endothelin receptor type B, tetratricopeptide repeat domain 3, WAP four-disulfide core domain 3, cytochrome P450 (family 1, subfamily B, polypeptide 1), p8 protein (candidate of metastasis 1), interferon gamma-inducible protein 16, dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2), solute carrier family 39 (zinc transporter), member 6, heat shock 70 kDa protein 2, vesicle-associated membrane protein 2 (synaptobrevin 2), Similar to AI661453 protein, and transient receptor potential cation channel (subfamily M, member 1), tyrosinase (oculocutaneous albinism IA), endothelin receptor type B, tetratricopeptide repeat domain 3, syndecan binding protein (syntenin), v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog, OTU domain, ubiquitin aldehyde binding 1, protein phosphatase 1 regulatory (inhibitor) subunit 12A, calponin 2, dishevelled dsh homolog 3 (Drosophila), tribbles homolog 2 (Drosophila), mucolipin 3, actinin alpha 4, ribosomal protein S15, CDC37 cell division cycle 37 homolog (S. cerevisiae), jumonji domain containing 3, v-maf musculoaponeurotic fibrosarcoma oncogene homolog B (avian), c-Maf-inducing protein, myosin heavy polypeptide 14, Hypothetical protein MGC40222, or combinations thereof. The kit may include one or more pairs of forward primers that selectively bind upstream of a gene on one strand and reverse primers that selectively bind upstream of a gene on a complementary strand. In another embodiment, the kit includes a microarray containing at least a fragment of a gene or a nucleic acid or protein product of a gene identified in any of Tables 1-6 or any combination thereof.

In another embodiment, the kit for characterizing a skin lesion in a subject includes an applicator and one or more probes or primers that selectively bind to one or more nucleic acid molecules in any of Tables 1-6, or to a nucleic acid or protein expression product of a nucleic acid molecule in any of Tables 1-6. In one embodiment, the probes are detectably labeled for visual identification of expression of RNA.

BRIEF DESCRIPTION OF THE DRAWINGS

FIGS. 1A and 1B are graphical diagrams showing data from the EDR, PTP, and PTN as a function of sample size, assuming a threshold for declaring the significance of a probe/gene expression difference between nevi and primary melanoma of p<0.05.

FIGS. 2A and 2B are graphical diagrams showing data from a sample size analysis that considered the contrast results for nevi vs. primary melanoma in the context of an analysis of variance (ANOVA) comparing normal skin, nevi, and primary melanoma

FIGS. 3A and 3B are graphical diagrams showing data from an analysis focusing exclusively on the posterior true probability (PTP) for different assumed significance levels.

FIGS. 4A to 4D are pictorial and graphical diagrams showing the development of a gene classifier for distinguishing melanoma from atypical nevi and normal pigmented skin.

FIGS. 5A and 5B are graphical diagrams showing data from prediction analysis of the developed classifiers for distinguishing melanoma from atypical nevi and normal pigmented skin.

FIGS. 6A to 6E are graphical diagrams showing data from prediction analysis of the developed classifiers for distinguishing melanoma from atypical nevi and normal pigmented skin.

DETAILED DESCRIPTION OF THE INVENTION

The present invention is based, in part, on the discovery that analysis of nucleic acid molecules or of protein expression products of nucleic acid molecules from specific genes can be used to characterize skin lesions in a subject. Accordingly, the present invention provides methods and kits useful for detecting cancer, especially melanoma by determining the expression profiles of one or more specific genes of interest.

There are two main motivations for conducting genome wide expression profiling studies in melanoma. First, melanoma is one of the best characterized carcinogenesis models for gradual progression of benign lesions to cancer: normal pigmented cells to nevi to atypical nevi to primary melanoma in situ to invasive primary melanoma to aggressive metastatic melanoma. This progression is known to correlate with distinctive chromosomal changes, and is thought to be mediated by stepwise progressive changes in gene expression, suggesting that expression profiling may identify genes responsible for tumorigenesis in melanoma. Indeed, candidate tumor genes have been identified with microarray analyses of melanoma cell lines. The second reason is that molecular characterization of tumors may allow a better staging classification of tumors and prognosis prediction. While histological characteristics such as the thickness and ulceration of tumors have some value as predictors of prognosis, there is lack of informative markers that help determine which patients will do well and which patients will have progressive disease and metastasis. Molecular markers identified in microarray experiments of tumors are already being introduced into clinical practice in the management of breast cancer. Gene expression profiling experiments in melanoma and melanoma cell lines suggest that the classification of melanoma can be improved, but studies are lacking with sufficient power to define molecular criteria for diagnosis or identify prognostic markers; the establishments of such markers would represent a major advance in melanoma care. A major reason for the lack of powerful microarray studies in melanoma is that, unlike most solid tumors, it is necessary to paraffin embed and section the whole lesion for histology, leaving no sample for RNA isolation. Although this situation is now changing, the ability to avoid biopsy until a definitive diagnosis is made would be powerful for subjects that would not normally be eligible for one or more biopsies.

As used in this specification and the appended claims, the singular forms “a”, “an”, and “the” include plural references unless the context clearly dictates otherwise. Thus, for example, references to “the method” includes one or more methods, and/or steps of the type described herein which will become apparent to those persons skilled in the art upon reading this disclosure and so forth.

Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the invention, the preferred methods and materials are now described.

The term “subject” as used herein refers to any individual or patient to which the subject methods are performed. Generally the subject is human, although as will be appreciated by those in the art, the subject may be an animal. Thus other animals, including mammals such as rodents (including mice, rats, hamsters and guinea pigs), cats, dogs, rabbits, farm animals including cows, horses, goats, sheep, pigs, etc., and primates (including monkeys, chimpanzees, orangutans and gorillas) are included within the definition of subject.

As used herein, the terms “sample” and “biological sample” refer to any sample suitable for the methods provided by the present invention. A sample of cells can be any sample, including, for example, a skin sample obtained by non-invasive tape stripping or biopsy of a subject, or a sample of the subject's bodily fluid. Thus, in one embodiment, the biological sample of the present invention is a tissue sample, e.g., a biopsy specimen such as samples from needle biopsy. In one embodiment, the term “sample” refers to any preparation derived from skin of a subject. For example, a sample of cells obtained using the non-invasive method described herein can be used to isolate nucleic acid molecules or proteins for the methods of the present invention. Samples for the present invention typically are taken from a skin lesion, which is suspected of being the result of a disease or a pathological or physiological state, such as psoriasis or dermatitis, or the surrounding margin or tissue. As used herein, “surrounding margin” or “surrounding tissue” refers to tissue of the subject that is adjacent to the skin lesion, but otherwise appears to be normal or free from lesion.

As used herein “corresponding normal cells” or “corresponding normal sample” refers to cells or a sample from a subject that is from the same organ and of the same type as the cells being examined. In one aspect, the corresponding normal cells comprise a sample of cells obtained from a healthy individual that does not have a skin lesion or skin cancer. Such corresponding normal cells can, but need not be, from an individual that is age-matched and/or of the same sex as the individual providing the cells being examined. Thus, the term “normal sample” or “control sample” refers to any sample taken from a subject of similar species that is considered healthy or otherwise not suffering from the particular disease, pathological or physiological state, or from the same subject in an area free from skin lesions. As such, a normal/standard level of RNA denotes the level of RNA present in a sample from the normal sample. A normal level of RNA can be established by combining skin samples or cell extracts taken from normal healthy subjects and determining the level of one or more RNAs present. In addition, a normal level of RNA also can be determined as an average value taken from a population of subjects that is considered to be healthy, or is at least free of a particular disease, pathological or physiological state. Accordingly, levels of RNA in subject, control, and disease samples can be compared with the standard values. Deviation between standard and subject values establishes the parameters for diagnosing or characterizing disease.

The term “skin” refers to the outer protective covering of the body, consisting of the epidermis (including the stratum corneum) and the underlying dermis, and is understood to include sweat and sebaceous glands, as well as hair follicle structures. Throughout the present application, the adjective “cutaneous” can be used, and should be understood to refer generally to attributes of the skin, as appropriate to the context in which they are used. The epidermis of the human skin comprises several distinct layers of skin tissue. The deepest layer is the stratum basalis layer, which consists of columnar cells. The overlying layer is the stratum spinosum, which is composed of polyhedral cells. Cells pushed up from the stratum spinosum are flattened and synthesize keratohyalin granules to form the stratum granulosum layer. As these cells move outward, they lose their nuclei, and the keratohyalin granules fuse and mingle with tonofibrils. This forms a clear layer called the stratum lucidum. The cells of the stratum lucidum are closely packed. As the cells move up from the stratum lucidum, they become compressed into many layers of opaque squamae. These cells are all flattened remnants of cells that have become completely filled with keratin and have lost all other internal structure, including nuclei. These squamae constitute the outer layer of the epidermis, the stratum corneum. At the bottom of the stratum corneum, the cells are closely compacted and adhere to each other strongly, but higher in the stratum they become loosely packed, and eventually flake away at the surface.

As used herein, the term “skin lesion” refers to a change in the color or texture in an area of skin. As such, “skin lesions suspected of being melanoma” are skin lesions with characteristics of malignant melanoma, which are well known to those of skill in the art, such as dermatologists and oncologists. Such lesions are sometimes raised and can have a color that is different from the color of normal skin of an individual (e.g., brown, black, red, or blue). Lesions suspected of being melanoma sometimes include a mixture of colors, are often asymmetrical, can change in appearance over time, and may bleed. A skin lesion suspected of being melanoma may be a mole or nevus. Melanoma lesions are usually, but not always, larger than 6 mm in diameter. Melanoma includes superficial spreading melanoma, nodular melanoma, acral lentiginous melanoma, and lentigo-maligna melanoma. Melanoma can occur on skin that has been overexposed to the sun. Therefore, in one embodiment the skin sample is taken from an area of skin that has been overexposed to the sun.

The term “dysplastic nevus” refers to an atypical mole or a mole whose appearance is different from that of common moles. Dysplastic nevi are generally larger than ordinary moles and have irregular and indistinct borders. Their color frequently is not uniform and ranges from pink to dark brown; they usually are flat, but parts may be raised above the skin surface. Dysplastic naevus can be found anywhere, but are most common on the trunk of a subject.

The term “cancer” as used herein, includes any malignant tumor including, but not limited to, carcinoma and sarcoma. Cancer arises from the uncontrolled and/or abnormal division of cells that then invade and destroy the surrounding tissues. As used herein, “proliferating” and “proliferation” refer to cells undergoing mitosis. As used herein, “metastasis” refers to the distant spread of a malignant tumor from its sight of origin. Cancer cells may metastasize through the bloodstream, through the lymphatic system, across body cavities, or any combination thereof. The term “cancerous cell” as provided herein, includes a cell afflicted by any one of the cancerous conditions provided herein. The term “carcinoma” refers to a malignant new growth made up of epithelial cells tending to infiltrate surrounding tissues, and to give rise to metastases. The term “melanoma” refers to a malignant tumor of melanocytes which are found predominantly in skin but also in bowel and the eye. “Melanocytes” refer to cells located in the bottom layer, the basal lamina, of the skin's epidermis and in the middle layer of the eye. Thus, “melanoma metastasis” refers to the spread of melanoma cells to regional lymph nodes and/or distant organs (e.g., liver, brain, breast, prostate, etc.).

As used herein, the term “gene” refers to a linear sequence of nucleotides along a segment of DNA that provides the coded instructions for synthesis of RNA, which, when translated into protein, leads to the expression of hereditary character. As such, the term “skin marker” or “biomarker” refers to a gene whose expression level is different between skin surface samples at the site of malignant melanoma and skin surface samples of normal skin or a lesion, which is benign, such as a benign nevus. Therefore, expression of a melanoma skin marker of the invention is related to, or indicative of, melanoma. Many statistical techniques are known in the art, which can be used to determine whether a statistically significant difference in expression is observed at a high (e.g., 90% or 95%) confidence level. As such, an increase or decrease in expression of these genes is related to and can characterize malignant melanoma. In one embodiment, there is at least a two-fold difference in levels between skin sample near the site of malignant melanoma and skin samples from normal skin.

As used herein, the term “nucleic acid molecule” means DNA, RNA, single-stranded, double-stranded or triple stranded and any chemical modifications thereof. Virtually any modification of the nucleic acid is contemplated. A “nucleic acid molecle” can be of almost any length, from 10, 20, 30, 40, 50, 60, 75, 100, 125, 150, 175, 200, 225, 250, 275, 300, 400, 500, 600, 700, 800, 900, 1000, 1500, 2000, 2500, 3000, 3500, 4000, 4500, 5000, 6000, 7000, 8000, 9000, 10,000, 15,000, 20,000, 30,000, 40,000, 50,000, 75,000, 100,000, 150,000, 200,000, 500,000, 1,000,000, 1,500,000, 2,000,000, 5,000,000 or even more bases in length, up to a full-length chromosomal DNA molecule. For methods that analyze expression of a gene, the nucleic acid isolated from a sample is typically RNA.

Micro-RNAs (miRNA) are small single stranded RNA molecules an average of 22 nucleotides long that are involved in regulating mRNA expression in diverse species including humans (reviewed in Bartel 2004). The first report of miRNA was that of the lin-4 gene, discovered in the worm C. elegans (Lee, Feinbaum et al. 1993). Since then hundreds of miRNAs have been discovered in flies, plants and mammals. miRNAs regulate gene expression by binding to the 3′-untranslated regions of mRNA and catalyze either i) cleavage of the mRNA; or 2) repression of translation. The regulation of gene expression by miRNAs is central to many biological processes such as cell development, differentiation, communication, and apoptosis (Reinhart, Slack et al. 2000; Baehrecke 2003; Brennecke, Hipfner et al. 2003; Chen, Li et al. 2004). Recently it has been shown that miRNA are active during embryogenesis of the mouse epithelium and play a significant role in skin morphogenesis (Yi, O'Carroll et al. 2006).

Given the role of miRNA in gene expression it is clear that miRNAs will influence, if not completely specify the relative amounts of mRNA in particular cell types and thus determine a particular gene expression profile (i.e., a population of specific mRNAs) in different cell types. In addition, it is likely that the particular distribution of specific miRNAs in a cell will also be distinctive in different cell types. Thus, determination of the miRNA profile of a tissue may be used as a tool for expression profiling of the actual mRNA population in that tissue. Accordingly, miRNA levels and/or detection of miRNA mutations are useful for the purposes of disease detection, diagnosis, prognosis, or treatment-related decisions (i.e., indicate response either before or after a treatment regimen has commenced) or characterization of a particular disease in the subject.

As used herein, the term “protein” refers to at least two covalently attached amino acids, which includes proteins, polypeptides, oligopeptides and peptides. A protein may be made up of naturally occurring amino acids and peptide bonds, or synthetic peptidomimetic structures. Thus “amino acid”, or “peptide residue”, as used herein means both naturally occurring and synthetic amino acids. For example, homo-phenylalanine, citrulline and noreleucine are considered amino acids for the purposes of the invention. “Amino acid” also includes imino acid residues such as proline and hydroxyproline. The side chains may be in either the (R) or the (S) configuration.

A “probe” or “probe nucleic acid molecule” is a nucleic acid molecule that is at least partially single-stranded, and that is at least partially complementary, or at least partially substantially complementary, to a sequence of interest. A probe can be RNA, DNA, or a combination of both RNA and DNA. It is also within the scope of the present invention to have probe nucleic acid molecules comprising nucleic acids in which the backbone sugar is other that ribose or deoxyribose. Probe nucleic acids can also be peptide nucleic acids. A probe can comprise nucleolytic-activity resistant linkages or detectable labels, and can be operably linked to other moieties, for example a peptide.

A single-stranded nucleic acid molecule is “complementary” to another single-stranded nucleic acid molecule when it can base-pair (hybridize) with all or a portion of the other nucleic acid molecule to form a double helix (double-stranded nucleic acid molecule), based on the ability of guanine (G) to base pair with cytosine (C) and adenine (A) to base pair with thymine (T) or uridine (U). For example, the nucleotide sequence 5′-TATAC-3′ is complementary to the nucleotide sequence 5′-GTATA-3′.

The term “antibody” as used in this invention is meant to include intact molecules of polyclonal or monoclonal antibodies, as well as fragments thereof, such as Fab and F(ab′)₂, Fv and SCA fragments which are capable of binding an epitopic determinant. The term “specifically binds” or “specifically interacts,” when used in reference to an antibody means that an interaction of the antibody and a particular epitope has a dissociation constant of at least about 1×10⁻⁶, generally at least about 1×10⁻⁷, usually at least about 1×10⁻⁸, and particularly at least about 1×10⁻⁹ or 1×10⁻¹⁰ or less.

As used herein “hybridization” refers to the process by which a nucleic acid strand joins with a complementary strand through base pairing. Hybridization reactions can be sensitive and selective so that a particular sequence of interest can be identified even in samples in which it is present at low concentrations. In an in vitro situation, suitably stringent conditions can be defined by, for example, the concentrations of salt or formamide in the prehybridization and hybridization solutions, or by the hybridization temperature, and are well known in the art. In particular, stringency can be increased by reducing the concentration of salt, increasing the concentration of formamide, or raising the hybridization temperature. For example, hybridization under high stringency conditions could occur in about 50% formamide at about 37° C. to 42° C. Hybridization could occur under reduced stringency conditions in about 35% to 25% formamide at about 30° C. to 35° C. In particular, hybridization could occur under high stringency conditions at 42° C. in 50% formamide, 5×SSPE, 0.3% SDS, and 200 mg/ml sheared and denatured salmon sperm DNA. Hybridization could occur under reduced stringency conditions as described above, but in 35% formamide at a reduced temperature of 35° C. The temperature range corresponding to a particular level of stringency can be further narrowed by calculating the purine to pyrimidine ratio of the nucleic acid of interest and adjusting the temperature accordingly. Variations on the above ranges and conditions are well known in the art.

As used herein, the term “mutation” refers to a change in the genome with respect to the standard wild-type sequence. Mutations can be deletions, insertions, or rearrangements of nucleic acid sequences at a position in the genome, or they can be single base changes at a position in the genome, referred to as “point mutations.” Mutations can be inherited, or they can occur in one or more cells during the lifespan of an individual.

As used herein, the term “kit” or “research kit” refers to a collection of products that are used to perform a biological research reaction, procedure, or synthesis, such as, for example, a detection, assay, separation, purification, etc., which are typically shipped together, usually within a common packaging, to an end user.

As used herein, the term “ameliorating” or “treating” means that the clinical signs and/or the symptoms associated with the cancer or melanoma are lessened as a result of the actions performed. The signs or symptoms to be monitored will be characteristic of a particular cancer or melanoma and will be well known to the skilled clinician, as will the methods for monitoring the signs and conditions. Thus, a “treatment regimen” refers to any systematic plan or course for treating a disease or cancer in a subject.

Samples from a tissue can be isolated by any number of means well known in the art. Invasive methods for isolating a sample include, but are not limited to the use of needles or scalpels, for example during biopsies of various tissues. Non-invasive methods for isolating a sample include, but are not limited to tape-stripping and skin scraping.

Accordingly, in one embodiment, the present invention employs a non-invasive tape stripping technology to obtain samples of suspicious lesions. As such, DNA microarray assays are used to create a non-invasive diagnostic for melanoma. Tape-stripping removes superficial cells from the surface of the skin as well as adnexal cells. Small amounts of nucleic acid molecules isolated from tape-stripped cells can be amplified and used for microarray analyses and quantitative PCR. In addition, proteins obtained from the lysed cells may be quantitated for diagnosis of disease. Consequently, tape-stripping is a non-invasive diagnostic method, which does not interfere with subsequent histological analyses, thereby bypassing a major limitation to current expression profiling studies on melanoma. While tape stripping will primarily sample superficial cells from the epidermis, this method holds great promise in the diagnoses and prognosis prediction in pigmented lesions for the following reasons: First, in contrast to benign nevi, in many melanomas the pigmented cells migrate into the epidermis and/or adnexa. Consequently, this feature may help differentiate benign pigmented lesions from melanomas based on tape stripping. Second, there are changes in the dermis and epidermis adjacent to melanoma. The epidermal hyperplasia overlying melanoma seems to correlate with both angiogenesis and metastatic potential; these changes are expected to be sampled with the tape stripping method. Finally, some advanced melanomas do reach the surface of the skin and melanoma cancer cells would be sampled directly by the tape stripping. In addition tape stripping is useful in the care of patients with multiple pigmented lesions where it is unpractical to biopsy each and every lesion. Accordingly, the present invention demonstrates that stratum corneum RNA, harvested by tape stripping with Epidermal Genetic Information Retrieval (EGIR) (see U.S. Pat. No. 6,949,338, incorporated herein by reference), can be used to distinguish melanoma from dysplastic nevi in suspicious pigmented lesions.

As indicated, the tape stripping methods provided herein typically involve applying an adhesive tape to the skin of a subject and removing the adhesive tape from the skin of the subject one or more times. In certain examples, the adhesive tape is applied to the skin and removed from the skin about one to ten times. Alternatively, about ten adhesive tapes can be sequentially applied to the skin and removed from the skin. These adhesive tapes are then combined for further analysis. Accordingly, an adhesive tape can be applied to and removed from a target site 10, 9, 8, 7, 6, 5, 4, 3, 2, or 1 time, and/or 10, 9, 8, 7, 6, 5, 4, 3, 2, or 1 adhesive tape can be applied to and removed from the target site. In one illustrative example, the adhesive tape is applied to the skin between about one and eight times, in another example, between one and five times, and in another illustrative example the tape is applied and removed from the skin four times.

The rubber based adhesive can be, for example, a synthetic rubber-based adhesive. The rubber based adhesive in illustrative examples, has high peel, high shear, and high tack. For example, the rubber based adhesive can have a peak force tack that is at least 25%, 50%, or 100% greater than the peak force tack of an acrylic-based tape such as D-SQUAME™. D-SQUAME™ has been found to have a peak force of 2 Newtons, wherein peak force of the rubber based adhesive used for methods provided herein, can be 4 Newtons or greater. Furthermore, the rubber based adhesive can have adhesion that is greater than 2 times, 5 times, or 10 times that of acrylic based tape. For example, D-SQUAME™ has been found to have adhesion of 0.0006 Newton meters, whereas the rubber based tape provided herein can have an adhesion of about 0.01 Newton meters using a texture analyzer. Furthermore, in certain illustrative examples, the adhesive used in the methods provided herein has higher peel, shear and tack than other rubber adhesives, especially those used for medical application and Duct tape.

Virtually any size and/or shape of adhesive tape and target skin site size and shape can be used and analyzed, respectively, by the methods of the present invention. For example, adhesive tape can be fabricated into circular discs of diameter between 10 millimeters and 100 millimeters, for example between 15 and 25 millimeters in diameter. The adhesive tape can have a surface area of between about 50 mm² and 1000 mm², between about 100 mm² to 500 mm² or about 250 mm².

In another embodiment, the sample is obtained by means of an invasive procedure, such as biopsy. Biopsies may be taken instead of or after tape stripping and are subjected to standard histopathologic analysis. Analysis of biopsy samples taken simultaneously with tape stripping samples may then be correlated with the data generated from one or more of analysis of selected lesion RNA samples by DNA microarray, correlation of gene expression data with histopathology, and creation of a candidate expression classifier for diagnosis of melanoma.

As used herein, “biopsy” refers to the removal of cells or tissues for analysis. There are many different types of biopsy procedures known in the art. The most common types include: (1) incisional biopsy, in which only a sample of tissue is removed; (2) excisional biopsy, in which an entire lump or suspicious area is removed; and (3) needle biopsy, in which a sample of tissue or fluid is removed with a needle. When a wide needle is used, the procedure is called a core biopsy. When a thin needle is used, the procedure is called a fine-needle aspiration biopsy. Other types of biopsy procedures include, but are not limited to, shave biopsy, punch biopsy, curettage biopsy, and in situ biopsy. In another embodiment, the skin sample is obtained by scraping the skin with an instrument to remove one or more nucleic acid molecules from the skin.

The skin sample obtained using the tape stripping method includes, epidermal cells including cells comprising adnexal structures. In certain illustrative examples, the sample includes predominantly epidermal cells, or even exclusively epidermal cells. The epidermis consists predominantly of keratinocytes (>90%), which differentiate from the basal layer, moving outward through various layers having decreasing levels of cellular organization, to become the cornified cells of the stratum corneum layer. Renewal of the epidermis occurs every 20-30 days in uninvolved skin. Other cell types present in the epidermis include melanocytes, Langerhans cells, and Merkel cells. As illustrated in the Examples herein, the tape stripping method of the present invention is particularly effective at isolating epidermal samples.

Nucleic acid molecules can also be isolated by lysing the cells and cellular material collected from the skin sample by any number of means well known to those skilled in the art. For example, a number of commercial products available for isolating polynucleotides, including but not limited to, RNeasy™ (Qiagen, Valencia, Calif.) and TriReagent™ (Molecular Research Center, Inc, Cincinnati, Ohio) can be used. The isolated polynucleotides can then be tested or assayed for particular nucleic acid sequences, including a polynucleotide encoding a cytokine. Methods of recovering a target nucleic acid molecule within a nucleic acid sample are well known in the art, and can include microarray analysis.

Nucleic acid molecules may be analyzed in any number of ways known in the art. For example, the presence of nucleic acid molecules can be detected by DNA-DNA or DNA-RNA hybridization or amplification using probes or fragments of the specific nucleic acid molecule. Nucleic acid amplification based assays involve the use of oligonucleotides or oligomers based on the nucleic acid sequences to detect transformants containing the specific DNA or RNA.

In one embodiment, analysis of the nucleic acid molecules includes genetic analysis is to determine the nucleotide sequence of a gene. Since a difference in length or sequence between DNA fragments isolated from a sample and those of known sequences are due to an insertion, deletion, or substitution of one or more nucleotides, the determination of nucleic acid sequences provides information concerning mutations which have absolute influence on the physiology of the disease state in the subject. These mutations may also include transposition or inversion and are difficult to detect by other techniques than direct sequencing. For example, it has recently been shown that the presence of the c-kit-activating mutation, L576P, is indicative of malignant melanomas (see Table 1). Accordingly, the methods of the present invention may be used to detect genetic mutations in one or more genes listed in Tables 1-6 for diagnosis and/or characterization of a skin lesion in a subject.

A variety of protocols for detecting and measuring the expression of nucleic acid molecules, using either polyclonal or monoclonal antibodies specific for the protein expression product are known in the art. Examples include enzyme-linked immunosorbent assay (ELISA), radioimmunoassay (RIA), and fluorescence activated cell sorting (FACS). These and other assays are described, among other places, in Hampton, R. et al. (1990; Serological Methods, a Laboratory Manual, APS Press, St Paul, Minn.) and Maddox, D. E. et al. (1983; J. Exp. Med. 158:1211-1216).

In another embodiment, antibodies that specifically bind the expression products of the nucleic acid molecules of the invention may be used to characterize the skin lesion of the subject. The antibodies may be used with or without modification, and may be labeled by joining them, either covalently or non-covalently, with a reporter molecule.

A wide variety of labels and conjugation techniques are known by those skilled in the art and may be used in various nucleic acid and amino acid assays. Means for producing labeled hybridization or PCR probes for detecting sequences related to the nucleic acid molecules of Tables 1-6 include oligolabeling, nick translation, end-labeling or PCR amplification using a labeled nucleotide. Alternatively, the nucleic acid molecules, or any fragments thereof, may be cloned into a vector for the production of an mRNA probe. Such vectors are known in the art, are commercially available, and may be used to synthesize RNA probes in vitro by addition of an appropriate RNA polymerase such as T7, T3, or SP6 and labeled nucleotides. These procedures may be conducted using a variety of commercially available kits (Pharmacia & Upjohn, (Kalamazoo, Mich.); Promega (Madison Wis.); and U.S. Biochemical Corp., Cleveland, Ohio). Suitable reporter molecules or labels, which may be used for ease of detection, include radionuclides, enzymes, fluorescent, chemiluminescent, or chromogenic agents as well as substrates, cofactors, inhibitors, magnetic particles, and the like.

PCR systems usually use two amplification primers and an additional amplicon-specific, fluorogenic hybridization probe that specifically binds to a site within the amplicon. The probe can include one or more fluorescence label moieties. For example, the probe can be labeled with two fluorescent dyes: 1) a 6-carboxy-fluorescein (FAM), located at the 5′-end, which serves as reporter, and 2) a 6-carboxy-tetramethyl-rhodamine (TAMRA), located at the 3′-end, which serves as a quencher. When amplification occurs, the 5′-3′ exonuclease activity of the Taq DNA polymerase cleaves the reporter from the probe during the extension phase, thus releasing it from the quencher. The resulting increase in fluorescence emission of the reporter dye is monitored during the PCR process and represents the number of DNA fragments generated. In situ PCR may be utilized for the direct localization and visualization of target nucleic acid molecules and may be further useful in correlating expression with histopathological finding.

Means for producing specific hybridization probes for nucleic acid molecules of the invention include the cloning of the nucleic acid sequences into vectors for the production of mRNA probes. Such vectors are known in the art, commercially available, and may be used to synthesize RNA probes in vitro by means of the addition of the appropriate RNA polymerases and the appropriate labeled nucleotides. Hybridization probes may be labeled by a variety of reporter groups, for example, radionuclides such as 32P or 35S, or enzymatic labels, such as alkaline phosphatase coupled to the probe via avidin/biotin coupling systems, and the like.

In order to provide a basis for the diagnosis or characterization of disease associated with expression of the nucleic acid molecules of the invention, a normal or standard profile for expression is established. Standard hybridization may be quantified by comparing the values obtained from subjects of known skin characterization (e.g., from subjects either having melanoma or having dysplastic nevi). Standard values obtained from such samples may be compared with values obtained from samples from subjects having skin lesions that are suspected of being melanoma. Deviation between standard and subject values is used to establish the presence of disease.

Accordingly, in one aspect of the invention, a non-invasive sampling method is provided for the characterization of skin lesion on the skin. In one embodiment, a sample set of pigmented skin lesions is created. Each sample consists of nucleic acid molecules recovered by tape stripping or biopsy sample of the superficial epidermis overlying the lesion. In addition to tape striping, a standard biopsy of the same lesion may also be performed, along with accompanying histology and diagnosis. Nucleic acid molecules recovered by tape stripping the superficial epidermis of normal skin will serve as a negative control.

In another aspect, the invention provides a method of distinguishing melanoma from dysplastic nevi and/or normal pigmented skin in a subject. In one embodiment, the method includes analyzing a nucleic acid molecule from one or more genes listed in any of Tables 1-6, or any combination thereof. A target area of the skin of a subject that suspected of being melanoma is assayed for expression of a large number of genes. Analyzing expression includes any qualitative or quantitative method for detecting expression of a gene, many of which are known in the art. The method can include analyzing expression of specific markers by measuring expression of the markers using a quantitative method, or by using a qualitative method. Non-limiting methods for analyzing polynucleotides and polypeptides are discussed below.

Methods of analyzing expression of a gene of the present invention can utilize a microarray, or other miniature high-throughput technology, for detecting expression of one or more gene products. Quantitative measurement of expression levels using such microarrays is also known in the art, and typically involves a modified version of a traditional method for measuring expression as described herein. For example, such quantitation can be performed by measuring a phosphor image of a radioactive-labeled probe binding to a spot of a microarray, using a phosphohor imager and imaging software.

In a related aspect, the invention provides a method for diagnosing various disease states in a subject by identifying new diagnostic markers, specifically the classification and diagnosis of melanoma. By identifying gene sets that are unique to a given state, these differences in the genetic expression can be utilized for diagnostic purposes. In one embodiment, the nucleic acid molecule is RNA, including messenger RNA (mRNA) that is isolated from a sample from the subject. Up-regulated and down-regulated gene sets for a given disease state may be subsequently combined. The combination enables those of skill in the art to identify gene sets or panels that are unique to a given disease state. Such gene sets are of immense diagnostic value as they can be routinely used in assays that are simpler than microarray analysis (for example “real-time” quantitative PCR). Such gene sets also provide insights into pathogenesis and targets for the design of new drugs.

A reference database containing a number of reference projected profiles is also created from skin samples of subjects with known states, such as normal (i.e., non-melanoma) and various skin cancer disease states. The projected profile is then compared with the reference database containing the reference projected profiles. If the projected profile of the subject matches best with the profile of a particular disease state in the database, the subject is diagnosed as having such disease state. Various computer systems and software can be utilized for implementing the analytical methods of this invention and are apparent to one of skill in the art. Exemplary software programs include, but are not limited to, Cluster & TreeView (Stanford, URLs: rana.1b1.gov or microarray.org), GeneCluster (MIT/Whitehead Institute, URL: MPR/GeneCluster/GeneCluster.html), Array Explorer (SpotFire Inc, URL: spotfire.com/products/scicomp.asp#SAE) and GeneSpring (Silicon Genetics Inc, URL: sigenetics.com/Products/GeneSpring/index.html) (for computer systems and software, see also U.S. Pat. No. 6,203,987, incorporated herein by reference).

In another aspect, the methods of the present invention involve in situ analysis of the skin lesion for characterization thereof. For in situ methods, nucleic acid molecules do not need to be isolated from the subject prior to analysis. In one embodiment, detectably labeled probes are contacted with a cell or tissue of a subject for visual detection of expressed RNA to characterize the skin lesion.

In another aspect, the methods of the present invention can also be useful for monitoring the progression of diseases and the effectiveness of treatments. For example, by comparing the projected profile prior to treatment with the profile after treatment. In one embodiment, the method characterizes a cancer as melanoma metastasis based on analysis of one or more nucleic acid molecules from Tables 1-6. It is known that in many cases, by the time a diagnosis of melanoma is established in a subject, metastasis has already occurred since melanomas contain multiple cell populations characterized by diverse growth rates, karyotypes, cell-surface properties, antigenicity, immunogenicity, invasion, metastasis, and sensitivity to cytotoxic drugs or biologic agents. Thus, the present invention may be used to characterize cancer of an organ as having metastasized from melanoma.

In a related aspect, the methods of the present invention can also be useful for determining an appropriate treatment regimen for a subject having a specific cancer or melanoma. Thus, the methods of the invention are useful for providing a means for practicing personalized medicine, wherein treatment is tailored to a subject based on the particular characteristics of the cancer in the subject. The method can be practiced, for example, by first determining whether the skin lesion is melanoma, as described above.

The sample of cells examined according to the present method can be obtained from the subject to be treated, or can be cells of an established cancer cell line of the same type as that of the subject. In one aspect, the established cell line can be one of a panel of such cell lines, wherein the panel can include different cell lines of the same type of disease and/or different cell lines of different diseases associated with expression of the genes of interest. Such a panel of cell lines can be useful, for example, to practice the present method when only a small number of cells can be obtained from the subject to be treated, thus providing a surrogate sample of the subject's cells, and also can be useful to include as control samples in practicing the present methods.

Once disease is established and a treatment protocol is initiated, the methods of the invention may be repeated on a regular basis to monitor the expression profiles of the genes of interest in the subject. The results obtained from successive assays may be used to show the efficacy of treatment over a period ranging from several days to months. Accordingly, another aspect of the invention is directed to methods for monitoring a therapeutic regimen for treating a subject having skin cancer. A comparison of the expression profile or mutations in the nucleic acid sequence of the nucleic acid molecule prior to and during therapy will be indicative of the efficacy of the therapy. Therefore, one skilled in the art will be able to recognize and adjust the therapeutic approach as needed.

The efficacy of a therapeutic regimen for treating a cancer over time can be identified by an absence of symptoms or clinical signs of the particular cancer in a subject at the time of onset of therapy. In subjects diagnosed as having the particular cancer, the efficacy of a method of the invention can be evaluated by measuring a lessening in the severity of the signs or symptoms in the subject or by the occurrence of a surrogate end-point for the disorder.

In addition, such methods may help identify an individual as having a predisposition for the development of the disease, or may provide a means for detecting the disease prior to the appearance of actual clinical symptoms. A more definitive diagnosis of this type may allow health professionals to employ preventative measures or aggressive treatment earlier thereby preventing the development or further progression of the cancer.

When performed in a high throughput (or ultra-high throughput) format, the methods of the invention can be performed on a solid support (e.g., a microtiter plate, a silicon wafer, or a glass slide), wherein cell samples and/or genes of interest are positioned such that each is delineated from each other (e.g., in wells). Any number of samples or genes (e.g., 96, 1024, 10,000, 100,000, or more) can be examined in parallel using such a method, depending on the particular support used. Where samples are positioned in an array (i.e., a defined pattern), each sample in the array can be defined by its position (e.g., using an x-y axis), thus providing an “address” for each sample. An advantage of using an addressable array format is that the method can be automated, in whole or in part, such that cell samples, reagents, genes of interest, and the like, can be dispensed to (or removed from) specified positions at desired times, and samples (or aliquots) can be monitored, for example, for expression products and/or mutations in the nucleic acid sequence of the nucleic acid molecules from any one of the genes listed in Tables 1-6.

Thus, the microarray can be used to monitor the expression level of large numbers of genes simultaneously (to produce a transcript image), and to identify genetic variants, mutations and polymorphisms. Polynucleotides used in the microarray may be oligonucleotides that are specific to a gene or genes of interest in which at least a fragment of the sequence is known or that are specific to one or more unidentified cDNAs which are common to a particular cell type, developmental or disease state. In order to produce oligonucleotides to a known sequence for a microarray, the gene of interest is examined using a computer algorithm which starts at the 5′ or more preferably at the 3′ end of the nucleotide sequence. The algorithm identifies oligomers of defined length that are unique to the gene, have a GC content within a range suitable for hybridization, and lack predicted secondary structure that may interfere with hybridization. In certain situations it may be appropriate to use pairs of oligonucleotides on a microarray. The “pairs” will be identical, except for one nucleotide which preferably is located in the center of the sequence. The second oligonucleotide in the pair (mismatched by one) serves as a control. The number of oligonucleotide pairs may range from two to one million. The oligomers are synthesized at designated areas on a substrate using a light-directed chemical process. The substrate may be paper, nylon or other type of membrane, filter, chip, glass slide or any other suitable solid support.

According to another aspect of the present invention, a kit is provided that is useful for detecting cancer in a cell or tissue, e.g., using the methods provided by the present invention for characterizing a skin lesion in a subject. In one embodiment, a kit of the invention includes a skin sample collection device and one or more probes or primers that selectively bind to one or more of the nucleic acid molecules in any of Tables 1-6. In another embodiment, the kit includes one or more applicators in addition to or instead of the skin sample collection device. Such applicators are useful for in situ analysis of gene expression on the skin of a subject. For example, an applicator may be used to apply detectably labeled probes for visual detection of expressed RNA to characterize the skin lesion.

In another embodiment, a kit of the invention includes a probe that binds to a portion of a nucleic acid molecule in any of Tables 1-6. In another embodiment, the kit further includes a microarray that contains at least a fragment of a gene or a nucleic acid molecule or a protein product of any one of the genes listed in Tables 1-6. In some embodiments, many reagents may be provided in a kit of the invention, only some of which should be used together in a particular reaction or procedure. For example, multiple primers may be provided, only two of which are needed for a particular application.

In another embodiment, the kit of the invention provides a compartmentalized carrier including a first container containing a pair of primers. The primers are typically a forward primer that selectively binds upstream of a gene on one strand, and a reverse primer that selectively binds upstream of a gene on a complementary strand. Optionally the kits of the present invention can further include an instruction insert, e.g. disclosing methods for sample collection using the sample collection device and/or exemplary gene expression profiles for comparison with the expression profile of the sample taken from the subject.

The following examples are provided to further illustrate the advantages and features of the present invention, but are not intended to limit the scope of the invention. While they are typical of those that might be used, other procedures, methodologies, or techniques known to those skilled in the art may alternatively be used.

EXAMPLE 1 RNA Quantitation and Profiling

The core hypothesis of this study is that the overlying epidermis of an early melanoma can be recovered with tape and that RNA contained within this sample is different than nearby epidermal RNA, i.e. that this RNA is diagnostic because of the underlying melanoma. Such a change in gene expression is documented for more advanced melanomas (McCarty et al., 2003) and is presumed to be true for early melanomas.

This study is divided into two separate phases, a sample collection and characterization phase (phase 1) and an RNA profiling phase (phase 2). In phase 1 the tape stripped specimens and biopsied sample collections were performed by the principal investigator or trained individuals delegated by the principal investigator to obtain the biopsy sample at various sites. All biopsies are subject to standard histopathologic analysis. The RNA profiling phase (Phase 2), includes, but is not limited to RNA purification and hybridization to DNA microarrays for gene expression profiling.

Materials and reagents. Adhesive tape was purchased from Adhesives Research (Glen Rock, Pa.) in bulk rolls. These rolls were custom fabricated into small circular discs, 17 millimeters in diameter, by Diagnostic Laminations Engineering (Oceanside, Calif.). Human spleen total RNA was purchased from Ambion (catalogue # 7970; Austin, Tex.). RNeasy RNA extraction kit was purchased from Qiagen (Valencia, Calif.). Reverse transcriptase, PCR primers and probes, and TaqMan Universal Master Mix, which included all buffers and enzymes necessary for the amplification and fluorescent detection of specific cDNAs, were purchased from Applied Biosystems (Foster City, Calif.). MELT total nucleic acid isolation system was purchased from Ambion (Austin, Tex.).

RNA isolation. RNA was extracted from tapes using either pressure cycling technology (PCT; Garrett, Tao et al. 2002; Schumacher, Manak et al. 2002) or MELT total nucleic acid system. Tapes were extracted in pairs by insertion into a PULSE™ tube (Pressure Biosciences, Gaithersburg, Md.) with 1.2 mls of buffer RLT (supplied in the Qiagen RNeasy kit). PULSE™ tubes were inserted into the PCT-NEP2017 pressure cycler and the sample was extracted using the following parameters: room temperature; 5 pressure cycles of 35 Kpsi with pressure held for 20 seconds at the top and bottom of each cycle. After pressure extraction the buffer was removed and used to process the remaining tapes used to strip that site; the buffer was then processed according to the standard Qiagen RNeasy protocol for the collection of larger RNAs (>200 nucleotides) by application to a purification column to which large RNA molecules (i.e. mRNAs) bind, while the column flow-through is saved for microRNA purification. The column flow-through, which contains miRNA separated from mRNA, is processed according to the Qiagen miRNA purification procedure (on the world wide web at qiagen.com/literature/protocols/pdf/RY20.pdf) to purify the microRNA. RNA from the 2 sites stripped on each subject was pooled to create a single sample from each subject.

RNA isolation using MELT total nucleic acid protocol. Tapes were extracted in a 2 ml eppendorf tube with 192 ml MELT buffer plus 8 ml of MELT cocktail and vortexed for 10 minutes at room temperature. The MELT lysates were transferred to the dispensed binding bead master mix after spinning down for 3 minutes at >10,000×g and washed with 300 ml of Wash Solution 1 and 2. RNAs were eluted in 100 ml of elution solution.

Quantitation of mRNA. Experimental data is reported as the number of PCR cycles required to achieve a threshold fluorescence for a specific cDNA and is described as the “C_(t)” value (Gibson, Heid et al. 1996; Heid, Stevens et al. 1996; AppliedBiosystems 2001). Quantitation of total RNA mass was performed as previously described (Wong, Tran et al. 2004). Briefly, RNA mass recovered from tapes is determined by using quantitative RT-PCR with reference to a standard curve (C_(t. actin) vs. log [RNA]; AppliedBiosystems 2001) created from commercially purchased human spleen total RNA. The average of 6 replicate C_(t. actin) values was used to calculate the concentration of RNA in a sample with reference to the standard curve.

RNA amplification and array hybridization. RNA was isolated by the Multi-Enzymatic Liquefaction of Tissue method (Ambion, Austin, Tex.) and amplified using the WT-Ovation pico amplification system (NuGen, San Carlos, Calif.). The amplified RNA was hybridized to Affymetrix U133 plus 2.0 microarray and data were processed and analyzed using R from Bioconductor.

Sample size. Sample size calculations are presented in Example 2. This analysis predicts that in order to find 25-40 genes with high predictive value (p<0.001) for discriminating benign nevi from melanoma then approximately 30 melanomas and 30 non-melanoma lesions are needed.

Preprocessing GeneChip Data. The image files from scanning the Affymetrix GeneChips with the Affymetrix series 3000 scanner will be converted using GCOS software (Affymetrix) to “CEL” format files. Normalization of CEL files will be carried out using software from the Bioconductor suite (on the world wide web at bioconductor.org). In particular, a robust multiarray analysis with adjustments for optical noise and binding affinities of oligonucleotide probes (Wu et al., 2006; and Wu et al., 2004) as implemented by the function “just.gcrma” in the “gcrma” package will be used to normalize the GeneChip Data.

Statistical Approach for Microarray Data Analysis. Two generic statistical problems are addressed in this proposal: (i) identifying genes that are differentially expressed in different classes of lesions (i.e. melanoma versus non-melanoma lesions) and (ii) forming (and evaluating) rules for classification of melanoma and non-melanoma lesions into groups based on gene expression data.

The most important grouping divides melanoma from non-melanoma on the basis of biopsy results. The methods that will be used to address the problems identified above are now standard in the statistical evaluation of microarray data (for reviews see Smyth et al., 2003; and Lee, 2004)). These methods have been applied by others to data from Affymetrix arrays to study gene expression in prostate cancer (Stuart et al., 2004), to characterize changes in gene expression subsequent to HIV infection (Mitchell et al., 2003), and to develop a high throughput genotyping platform (Wolyn et al., 2004; and Borevitz et al., 2003). For identifying differentially expressed genes, permutation based estimates of false discovery rates (reviewed in Efron et al., 2002) are preferred. Scripts for the R quantitative programming environment were developed to implement these methods in our previous work, but will likely use or adapt the “siggenes” package from the Bioconductor suite in this project. The development of classification rules will rely on resampling methods (k-fold cross-validation, the 632 plus bootstrap, and/or bagging (Hastie et al., 2001) applied to the naive Bayes classifier and the nearest shrunken centroid classifier (Tibshirani et al., 2002) and the support vector machine (SVM) which both performed well in classifying prostate tissues as malignant or benign, used in our previous work. The implementation likely to be used is to perform k-fold cross-validation. Within each of the k train/test cycles an initial screen of the training data for differentially expressed genes is performed and genes are ordered according to their posterior probability of differential expression. Naive Bayes and nearest shrunken centroid classifiers based on the r genes with the highest posterior probability of differential expression are formed choosing enough values of r between 1 and 1024 to allow accurate interpolation of the classification error rate. The “one se rule” (Brieman et al., 1984) is applied to the error rates for the test sets to choose the classifier that minimizes the error rate. For SVM, an internal 632+ bootstrap is applied to each training sample to select the number of genes to be used in forming the classifier. The “1 se rule” error rates from the k test sets are used to characterize the classification accuracy.

In addition to the use of univariate and multivariate statistical analysis tools, sophisticated bioinformatic analysis approaches will help make sense of possible biological links between the genes found to be differentially expressed between, e.g., melanoma and non-melanoma samples. These approaches will focus on the analysis of genetic networks and pathways (Edelman et al., 2006; Kong et al., 2006; and Pang et al., 2006) and have been implemented in software packages such as Ingenuity (on the world wide web at ingenuity.com) and MetaCore (on the world wide web at genego.com). The identification of the biological links between genes that emerge from a gene expression microarray analysis can help put into context the biological meaningfulness of their expression patterns as well as help reduce the set of differentially expressed genes to be represented on a diagnostic panel based on their biology. The end result of this analysis will be to define a candidate expression classifier that will be validated in future, larger clinical trials.

QC metrics for RNA, amplified cDNA and microarray data. Following informed consent, the suspicious pigmented lesion was tape stripped using EGIR and then biopsied as per standard of care. The resulting RNA isolated from the EGIR tape was amplified and profiled on the Affymetrix U133 plus 2.0 GeneChip. Microarray data were normalized by the GCRMA algorithm. To assure high quality of microarray data are generated, QC metrics were established for RNA, amplified cDNA and microarray data. The quality of RNA was assessed by capillary electrophoresis using the Experion system (Biorad, Hercule, Calif.) and RNA with at least one visible 18S rRNA was further processed for RNA amplification. The amplified cDNA was quantified by the Nanodrop system and quality of the amplified cDNA was also assessed by the Experion system. The yield of the amplified cDNAs greater than 5 mg and the average size distribution of the cDNAs greater than 750 nt were carried forward for microarray hybridization. Quality of the array data was further assessed using simpleaffy program in R and the array data with scaling factor less than 5.0 and % present call greater than 30% were used for further data analysis.

Melanomas distinguished from dysplastic nevi and normal skin. After passing the array data QC, 14 melanomas, 40 dysplastic nevi and 12 normal skin specimens were further analyzed. First, gene expression values less than 50 across all samples were filtered out and 16716 probesets were tested. These 16716 probesets were subjected to a statistical analysis for differentially expressed genes among melanomas, dysplastic nevi and normal skin using ANOVA (p<0.05), multiple testing correction algorithm (Westafall and Young permutation) and false discover rate (FDR) of 0.05. As indicated above, of the original 117 genes, an 89 gene panel (Table 2) was found to be a potential melanoma classifier. Further testing identified a 5-gene classifier (Table 3), a 30-gene classifier (Table 4) that includes newly identified genes, a 20-gene classifier (Table 5) that includes newly identified genes, and a 19-gene classifier that includes newly identified genes, which may all be used to discriminate melanomas from atypical nevi. The genes and respective classifier panels were analyzed using the Prediction Analysis of Microarrays (PAM) software freely available from Stanford University (Stanford, Calif.).

The PAM software uses a modification of the nearest centroid method, which computes a standardized centroid for each class in a training set. This refers to the average gene expression for each gene in each class divided by the within-class standard deviation for that gene. Nearest centroid classification takes the gene expression profile of a new sample, and compares it to each of these class centroids. The class, whose centroid it is closest to, in squared distance, is the predicted class for that new sample.

These genes were all subjected to a hierarchical clustering analysis and the melanoma specimens grouped together and were clearly distinguished from dysplastic nevi and normal skin. In addition, there are three distinct classes of dysplastic nevi; one is grouped together with normal skin and the second one was in between normal skin and melanomas, while the third one was grouped together with melanomas. These data suggest stratum corneum RNA, harvested by tape stripping with EGIR, can be used to distinguish melanoma from dysplastic nevi in suspiciously pigmented lesions.

The analysis of the genes as potential melanoma classifiers to discriminate between melanomas and dysplastic nevi was performed using t-test (p<0.01), FDR (0.05) and 2-fold difference between melanomas and dysplastic nevi. Of the original 117 genes, an 89 gene panel (Table 2) was found to be a potential melanoma classifier and functions of these 89 genes were subjected to Ingenuity Pathway Analysis (IPA) (Ingenuity, Redwood City, Calif.). Among them, 15 genes are involved hair and skin development and function, 18 genes are involved in cellular development, 16 genes are involved in cellular growth and proliferation and 24 genes are related to cancer. Thus, differentially expressed genes are genes related to biological functions in melanocytes including melanin biosynthesis, melanocyte proliferation, differentiation and development. (See FIGS. 5 and 6).

EXAMPLE 2 Preliminary Power and Sample Size Studies Nevi Vs. Primary Melanoma

The following sample size and power calculations are based exclusively on the large-scale cDNA study data provided in Haqq et al (2005). That data focused on normal skin (n=3 samples), nevi (n=9), primary melanomas (n=6) and metastatic melanomas (n=19). For purposes of the sample size calculations, the focus was on the comparison of nevi to primary melanomas. Power and sample size assessments were calculated based on the bootstrap strategy outlined by Page et al. Using the raw data available from the Haqq et al (2005) study, gene expression differences—based on all 14,772 probes used in their cDNA assay—between nevi and primary melanomas were computed using simple t-tests for each probe/gene. Note that multiple probes can be used interrogate individual genes. In addition, normal skin, nevi, and primary melanoma gene expression differences were also assessed in a three group analysis of variance (ANOVA), with the specific contrast between nevi and primary melanoma computed from this ANOVA. In the figures that follow, three main parameters are used to assess power and sample size. Table 7 (adapted from Page, et al.) shows the number of genes truly or not truly differentially expressed, and provides a simple way of describing these parameters, which are defined as follows (with the color of the curves corresponding to each parameter provided in parentheses for FIGS. 1 a and 2 a, although FIGS. 1 b and 2 b focus exclusively on the EDR as defined below.

EDR (Blue line): Expected Discovery Rate (from Table 7, D/(B+D)). This reflects the expected proportion of probes/genes that will be declared significantly differentially expressed at the defined threshold (here taken to be, for the most part, p<0.05) that are, in fact, differentially expressed between nevi and primary melanomas.

PTP (Red line): Expected Proportion of probes/genes that are True Positives (Table 7, D/(C+D)). This proportion reflects the number of probes/genes showing expression differences that are likely to be truly differential expressed out of the total number of genes whose expression values result in test statistics less than the threshold (e.g., 0.05).

PTN (Green line): Probability of a True Negative result (Table 7, A/(A+B)). This probability concerns probes/genes that are not significantly different at the assumed threshold (e.g., 0.05) that are, in fact, not differentially expressed between skin and melanoma.

TABLE 7 Parameters of Relevance for Assessing the Power of Microarray Studies Not differentially Truly differentially Result based on array analysis expressed expressed Genes not significant A B Genes significant C D These columns represent the number of genes found to satisfy the given constraint; A = genes found not to be differentially expressed in an array experiment and that are truly not differentially expressed; B = genes that are differentially expressed but are not found to be differentially expressed in the array experiment (false negatives); C = genes that are found to be differentially expressed in the array experiment but are not truly differentially expressed (false positives); D = gene found to be differentially expressed in an array experiment and that are truly differentially expressed.

Nevi versus Primary data. The sample size analysis considered the number of samples necessary to “discover” or identify a probe or gene or set of probes/genes that could differentiate nevi from primary melanomas based on the probe/gene expression differences obtained by Haqq et al. (2005). FIG. 1 a provides a plot of the EDR, PTP, and PTN as a function of sample size, assuming a threshold for declaring the significance of a probe/gene expression difference between nevi and primary melanoma of p<0.05. Thus, from the plot, it appears that in order to “discover,” or identify, 80% of all genes that have been interrogated on a chip that exhibit a probe/gene expression difference producing a test statistic p-value <0.05 that will actually reflect a true probe/gene expression difference, a sample size of roughly 20 per nevi and primary melanoma group will be needed. Note that if all 14,772 probes are considered, one is likely to have 14,772×0.05=738 exhibit p-values <0.05 by chance alone, of which 1,727×0.80=1,381 will likely reflect true gene expression differences at that significance (i.e., p-value) level. If one is interested in identifying a smaller set of genes that have a greater probability of being detected as truly differentially expressed, a more stringent threshold for statistical significance (e.g., 0.001) can be used. This would generate 14,772×0.001=15 genes with p-values <0.001 by chance of which ˜45% (i.e., 34×0.45=7 would likely be truly differentially expressed at that level; see FIG. 1 b; note curves in FIG. 1 b only correspond to the EDR with different assumed type I error rates).

A sample size analysis that considered the contrast results for nevi vs. primary melanoma in the context of an analysis of variance (ANOVA) comparing normal skin, nevi, and primary melanoma was also pursued. The rationale for this is that there are more differences between normal skin and either nevi or primary melanoma than there are between nevi and primary melanoma (based on an analysis of the Haqq et al (2005) data), and an analysis that considers normal skin gene expression variation may help reduce the noise in the assessment of nevi vs. primary melanoma gene expression differences. FIGS. 2 a and 2 b display the results of these analyses and provide similar sample size guidelines to those reflected in FIGS. 1 a and 1 b.

An analysis focusing exclusively on the posterior true probability (PTP) was also considered since, as discussed, there may be many probes/genes that exhibit differences between nevi and primary melanomas at a certain probability level purely by chance (given the large number of probes/genes interrogated). Thus, the likely fraction of these probes/genes that are truly differentially expressed is important to assess. FIGS. 3 a and 3 b reflect the results for different assumed significance levels.

Thus, an argument can be made that a study with approximately 20 samples per nevi and primary melanoma groups would have sufficient power to detect 80% of all genes that are likely to exhibit differential expression at a p-value level of 0.05 because they are, in fact, differentially expressed at this level. However, the number of genes (or probes) contributing to this set of differentially expressed genes is likely to number in the hundreds, if 10,000-30,000 probes are used or 5,000-10,000 genes are studied. If interest is in identifying a smaller number of probes or genes (˜25-40) that have a greater probability of being differentially expressed, say, at a p-value of 0.001, then ˜30 nevi and 30 primary melanoma samples would be needed (see FIGS. 1, 2, and 3).

EXAMPLE 3 Tape Stripping to Recover Nucleic Acids from Normal Skin

The following procedure was used to recover nucleic acids from normal skin (e.g., the mastoid or upper back areas) of a subject.

Tapes were handled with gloved hands at all times. Locate a particular site that is relatively blemish-free and healthy, unless otherwise specified by the protocol. Preferred normal skin sites are the mastoid process (the bony process behind the ear at the base of the skull) and the upper back, immediately superior to the scapular spine. Shave the site if necessary to remove non-vellus hairs. Cleanse the site with an alcohol wipe (70% isopropyl alcohol). Let the site air dry completely before application of the tape. It is recommended to wait approximately 2 minutes to ensure the site is completely dry before application of the tape.

Apply the tape to the skin site. If more than one tape is used, apply tapes in sequential order starting from the left side. Use a surgical skin marker and/or a water soluble marker to mark the location of the tape on the skin in order to align subsequent tapes.

Start the tape harvesting procedure by applying pressure (press on the tape firmly). Ensure that the skin is held taut to ensure that the tape does not move while applying pressure. Then remove the tape slowly in one direction. Place the edge of the tape onto the strip at the top of the packet with the adhesive surface of the tape facing down to protect the sample. Put a second tape on the same site; apply pressure firmly as above. Remove the tape slowly in an opposite direction to that used in the immediately previous application.

Continue tape stripping by putting additional tapes on the same site, following the steps provided above. The site may stripped with a total of at least four tapes, unless otherwise specified in the protocol. Place the strip into a storage bag and immediately place the samples on dry ice or into storage at −20° C. or below until analysis.

EXAMPLE 4 Tape Stripping to Recover Nucleic Acids from Pigmented Lesions

The following procedure was used to recover nucleic acids from pigmented lesions and/or skin suspected of melanoma of a subject. In contrast to normal skin, lesional skin should have a preoperative biopsy diameter of greater than or equal to about 6 mm, but less than that of the tape disc. Multiple lesions must be at least about 4 mm apart. The area of tape that touches the lesion should be generously demarcated on the tape with an insoluble ink pen so that this area may be cut away from the surrounding tape at the laboratory as part of the RNA extraction procedure.

As above, tapes were handled with gloved hands at all times. Shave the site if necessary to remove non-vellus hairs. Cleanse the site with an alcohol wipe (70% isopropyl alcohol). Let the site air dry completely before application of the tape. It is recommended to approximately 2 minutes to ensure the site is completely dry before application of the tape.

Apply the tape to the skin site. If more than one tape is used, apply tapes in sequential order starting from the left side. Use a surgical skin marker and/or a water soluble marker to mark the location of the tape on the skin in order to align subsequent tapes. Apply the tape to the suspect lesion, which should have a diameter that is greater than or equal to about 6 mm.

Start the tape harvesting procedure by applying pressure directly over the lesion and avoiding surrounding normal skin (press on the tape firmly). Ensure that the skin is held taut to ensure that the tape does not move while applying pressure. Using a marking pen, demarcate a zone around the lesion such that the area of the lesion is encompassed within the inked boundary and the boundary is approximately 1 mm from the lesion border.

Remove the tape slowly in one direction. Place the edge of the tape onto the adhesive strip with cells facing down to protect the sample. Put a second tape on the same site following directions provided above. Repeat until the lesion has been stripped a total of at least four times, unless otherwise specified in the protocol. Place the strip into a storage bag and immediately place the samples on dry ice or into storage at −20° C. or below until analysis.

EXAMPLE 5 Gene Expression Profile to Distinguish Melanoma from Atypical Nevi

The purpose of this study is to determine whether stratum corneum RNA, harvested by tape stripping with EGIR can be used to distinguish melanoma from atypical nevi in suspicious pigmented lesions. See FIG. 4A.

Suspicious pigmented lesions were tape stripped four times using EGIR and then biopsied as per standard of care. Normal, uninvolved skin was tape stripped to serve as a negative control. All biopsies underwent primary and central review for histopathology. Total RNA was isolated from the tapes using MELT (Ambion, Inc.) and assessed for quality by Experion (Bio-Rad, Inc.) analysis. The yield of RNA was approximately 1 ng, as determined by quantitative RT-PCR of the specimen for β-actin gene expression. Total RNA (200-500 pg) was then amplified using the WT-Ovation Pico RNA Amplification System (NuGen, Inc.) and assayed for gene expression profile using the U133 plus 2.0 GeneChip (Affymetrix, Inc.).

The resulting RNA isolated from the EGIR tape is then amplified and profiled on the Affymetrix U133 plus 2.0 GeneChip. Microarray data is normalized by the GCRMA algorithm. Further analyses by means of ANOVA analysis (p<0.05) with a false discovery rate of 0.05 and multiple correction testing using Westfall and Young permutation identified approximately 117 genes as differentially expressed between melanoma, dysplastic nevi and normal skin (Table 1). Hierarchical clustering of these genes showed that the melanoma specimens grouped together and were clearly distinguished from dysplastic nevi and normal skin (FIG. 4B). In addition, 89 of the 117 genes shown in Table 1 were further identified (Table 2) as potential discriminators between melanoma and dysplastic nevi (p<0.01, false discovery rate q<0.05). When these 89 genes were subjected to Ingenuity Pathways analysis many were found to play roles in melanoma, hair and skin development and function, cellular development, cellular growth and proliferation and cancer. These findings demonstrate that EGIR-harvested RNA from suspicious pigmented skin lesions can be used to differentiate melanoma from dysplastic nevi (FIG. 4C). Further, these results suggest that the gene expression profile of stratum corneum is altered, either directly or indirectly, by the presence of melanoma (FIG. 4D).

In subsequent studies that compared normal and inflamed skin, sequential application of four small tapes at the same skin site recovered enough intact RNA to perform quantitative reverse-transcription polymerase chain reaction (qPCR) assay and DNA microarray analysis for investigation of gene expression. The latter assay was performed using the Affymetrix HG-U133A GeneChip following two rounds of amplification of 10 ng of total RNA sample that produced 30-80 μg of anti-sense RNA. Comparison of results from two subjects, each sampled at three separate sites, showed 12% intra- and inter-subject variance in gene measurements, a result that is well within the Affymetrix specified coefficient of variation (CV) for GeneChip assay. Of note is that differential expression of Y-chromosome genes was observed, a result that accurately distinguished the different genders of the 2 subjects. GeneChip assay was then performed on RNA isolated from tape stripping each of 3 subjects from normal, water occluded, and sodium lauryl sulfate-irritated study groups. The majority of 100 genes, whose expression is most significantly altered between untreated and SLS-treated skin showed, were already known to be involved in tissue inflammation and injury functions. Thus, RNA harvested by EGIR technology is more than adequate for microarray-based gene expression profiling and appropriately reflects the pathologic state of skin.

Recent work by Benson et al (2006) demonstrates that RNA can be recovered from psoriatic lesions and that the general RNA expression profile of tape strip recovered RNA is consistent with biopsy RNA derived from lesions on the same patient. Further work (see U.S. Pat. No. 7,183,057, incorporated herein by reference) has shown that psoriatic lesions can be sampled with tape during treatment with Enbrel and that strong correlations could be made between gene expression in week one of treatment and clinical response at weeks 4 and 8. This work further establishes the credentials of tape stripping for the recovery of physiologically relevant RNA from the surface of the skin.

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TABLE 1 Entrez Entrez Gene ID Gene ID for for Entrez Gene ID name matched term synonym description Human Mouse for Rat ACTR1B 202135_s_at 2310066K23Rik, ARP1 actin-related 10120 226977 (includes AA960180, protein 1 homolog B, EG: 10120) ACTR1B, centractin beta (yeast) AI851923, ARP1B, CTRN2, MGC36526 ANGEL1 213099_at 1110030H02Rik, angel homolog 1 23357 68737 362765 KIAA0759, (Drosophila) mKIAA0759, RGD1306238 ANKRD13B 227720_at AW124583, ankyrin repeat domain 124930 268445 360575 B930093C12Rik, 13B FLJ20418, FLJ25555, RGD1564005 ANKRD44 228471_at 4930444A19Rik, ankyrin repeat domain 44 91526 329154 301415 A130096K20, E130014H08Rik, LOC91526, MGC21968, MGC70444, RGD1561893 ARHGEF19 226857_at 6030432F23, Rho guanine nucleotide 128272 213649 362648 6430573B13Rik, exchange factor (GEF) 19 FLJ33962, RP4- 733M16.1, WGEF ATPBD4 238662_at 5730421E18Rik, ATP binding domain 4 89978 66632 362191 MGC14798, RGD1310006 BARX2 210419_at 2310006E12Rik, BarH-like homeobox 2 8538 12023 Barx2b, MGC133368, MGC133369 BDNF 206382_s_at MGC105254, brain-derived 627 12064 24225 MGC34632 neurotrophic factor BLOC1S1 202592_at AI839753, biogenesis of lysosome- 2647 14533 288785 BLOC-1 subunit related organelles 1, BLOS1, complex-1, subunit 1 GCN5-like protein 1, GCN5L1, MGC87455, RT14 BTG2 201236_s_at AA959598, Agl, BTG family, member 2 7832 12227 29619 An, an-1, APRO1, MGC126063, MGC126064, PC3, TIS21 C16ORF48 223407_at AI606951, chromosome 16 open 84080 102124 291975 DAKV6410, reading frame 48 DKFZP434A1319, E130303B06Rik, RGD1307357 C6ORF218 244829_at MGC40222 chromosome 6 open 221718 reading frame 218 C8ORF13 233641_s_at A030013D21, chromosome 8 open 83648 219148 498533 BC065085, reading frame 13 D8S265, DKFZp761G151, MGC120649, MGC120650, MGC120651, RGD1561302 CCDC95 227286_at AI225782, coiled-coil domain 283899 233875 AI854876, containing 95 Ccdc85, FLJ00079, FLJ90652, MGC31515 CCHCR1 37425_g_at C6orf18, HCR, coiled-coil alpha-helical 54535 240084 406196 MGC126371, rod protein 1 MGC126372, MGC28303, RGD: 1302992, SBP CIRBP 230142_s_at A18 HNRNP, cold inducible RNA 1153 12696 81825 CIRP, R74941 binding protein CLSTN2 219414_at 2900042C18Rik, calsyntenin 2 64084 64085 171394 AI448973, alcagamma, CS2, Cst-2, CSTN2, FLJ39113, FLJ39499, KIAA4134, MGC119560, mKIAA4134 COL7A1 217312_s_at AW209154, collagen, type VII, alpha 1294 12836 301012 EBD1, EBDCT, 1 (epidermolysis bullosa, EBR1 dystrophic, dominant and recessive) DACH1 205471_s_at, AI182278, Dac, dachshund homolog 1 1602 13134 205472_s_at, DACH, (Drosophila) 228915_at E130112M23Rik, FLJ10138 DCT 205337_at, DT, dopachrome tautomerase 1638 13190 290484 205338_s_at RGD1564975, (dopachrome delta- slaty, slt, TRP-2, isomerase, tyrosine-related TYRP2 protein 2) DOCK10 219279_at 9330153B10RIK, dedicator of cytokinesis 55619 210293 301556 A630054M16Rik, 10 DKFZp781A1532, DRIP2, Jr4, Jr5, mKIAA0694, Nbla10300, R75174, RGD1561963, ZIZ3, Zizimin3 DRAP1 1556181_at 2310074H19Rik, DR1-associated protein 1 10589 66556 293674 MGC156767, (negative cofactor 2 alpha) NC2-ALPHA, negative cofactor 2 alpha EDNRB 204271_s_at, ABCDS, endothelin receptor type B 1910 13618 50672 206701_x_at AU022549, Ednra, ET&gt; B&lt;, ET-B, ETB RECEPTOR, ETBR, ETRB, GUSB, HSCR, HSCR2, Sox10m1 EFNA4 205107_s_at EFL-4, EPHRIN ephrin-A4 1945 13639 310643 A4, Epl4, EPLG4, LERK-4, MGC125826 EHD2 45297_at BC027084, EH-domain containing 2 30846 259300 361512 C130052H20Rik, MGC25606, MGC38650, MGEPS, PAST2 ETS1 224833_at AI196000, v-ets erythroblastosis 2113 23871 24356 AI448617, C- virus E26 oncogene ETS1, homolog 1 (avian) D230050P06, Etsoncb, EWSR2, FLJ10768, MGC124638, MGC130355, MGC18571, p42 ETS1, p51 ETS1, Tpl1 FAM33A 225684_at 1110001A07Rik, family with sequence 348235 66140|625534 287598 C78640, similarity 33, member A EG625534, FLJ12758, MGC109093, MGC110975, MGC151378, RGD1307084 FGFR1 210973_s_at, AW208770, fibroblast growth factor 2260 14182 79114 211535_s_at BFGFR, C-FGR, receptor 1 (fms-related CD331, CEK, tyrosine kinase 2, Pfeiffer FGF1 syndrome) RECEPTOR, FGFBR, FGFR1- IIIC, Fgfr1c, FLG, Flk2, FLT2, H5, HBGFR, KAL2, N-SAM FOXO1A 202723_s_at Afxh, AI876417, forkhead box O1A 2308 56458 84482 FKH1, FKHR, (rhabdomyosarcoma) FKHR1, Forkhead, FOXO1 FOXP1 223936_s_at 12CC4, forkhead box P1 27086 108655 297480 3110052D19Rik, 4932443N09Rik, AI461938, AW494214, FLJ23741, hFKH1B, HSPC215, MGC116362, MGC12942, MGC88572, MGC99551, QRF1 FRAT2 209864_at MGC10562, frequently rearranged in 23401 212398 MGC37615 advanced T-cell lymphomas 2 GCLM 203925_at Gamma gclm, glutamate-cysteine ligase, 2730 14630 29739 Gamma modifier subunit glutamylcysteine synthase (regulatory), GAMMA GLUTAMYLCYSTEINE SYNTHETASE, Gcs Ls, Gcs, Regulatory, GCS- L, GCS1, Gcslc, GLCLR, glutamat-cystein ligase, regulatory subunit GGA3 209411_s_at C230037M19Rik, golgi associated, gamma 23163 260302 360658 KIAA0154, adaptin ear containing, mKIAA0154 ARF binding protein 3 GLUL 200648_s_at GLNS, glutamate-ammonia 2752 14645 Glutamine ligase (glutamine Synthase, synthetase) GLUTAMINE SYNTHETASE, GS, MGC128403, PIG43 GPR161 214104_at FLJ33952, G- G protein-coupled 23432 240888 289180 protein coupled receptor 161 receptor af091890, Gm208, Gm208Gpr, RE2, RGD1563245 HEY2 219743_at CHF1, GRL, hairy/enhancer-of-split 23493 15214 155430 HERP1, HESR2, related with YRPW motif 2 HRT2, MGC10720 HIST2H2AA3 214290_s_at AI448581, H2A, histone cluster 2, H2aa3 8337 15267 365877 H2a-615, H2A.2, H2A/O, H2A/q, H2AFO, Hist2, HIST2H2AA, Hist2h2aa1 ID1 208937_s_at AI323524, inhibitor of DNA binding 3397 15901 25261 D2Wsu140e, ID, 1, dominant negative ID-1H, ID125A, helix-loop-helix protein Idb1, MGC156482 KALRN 227750_at 2210407G14Rik, kalirin, RhoGEF kinase 8997 545156 84009 AV235988, DUET, Duo, E530005C20Rik, FLJ16443, Gm539, HAPIP, KALIRIN, Kalirin7, Pcip10, TRAD KDELR1 200922_at 8030486F04Rik, KDEL (Lys-Asp-Glu- 10945 68137 361577 AW215843, Leu) endoplasmic ERD2, ERD2.1, reticulum protein retention HDEL, KDEL receptor 1 RECEPTOR, Kdelr, MGC109169, PM23 KIAA0738 210529_s_at 2810407D09Rik, KIAA0738 gene product 9747 77574 362353 3321401G04Rik, A230020K05Rik, AI848529, RGD1565474 KIT 205051_s_at Bs, C-KIT, c-Kit v-kit Hardy-Zuckerman 4 3815 16590 64030 Gnnk+, CD117, feline sarcoma viral Fdc, SCFR, Ssm, oncogene homolog Tr Kit, white- spotted LGR4 230674_at 9130225G07, leucine-rich repeat- 55366 107515 286994 A930009A08Rik, containing G protein- GPCR48, GPR48 coupled receptor 4 LHX2 211219_s_at ap, apterous, LIM homeobox 2 9355 16870 296706 (includes hLhx2, Lh-2, EG: 9355) LH2A, Lhx2, Lim2, MGC138390 LMO4 209204_at A730077C12Rik, LIM domain only 4 8543 16911 362051 Crp3, Etohi4, MGC105593 LOC254100 1557131_at hypothetical protein 254100 LOC254100 LRIG1 236173_s_at, D6Bwg0781e, leucine-rich repeats and 26018 16206 312574 238339_x_at DKFZP586O1624, immunoglobulin-like Img, LIG-1 domains 1 MED28 222635_s_at 1500003D12Rik, mediator of RNA 80306 66999 305391 AI451633, polymerase II AU045690, transcription, subunit 28 DKFZP434N185, homolog (S. cerevisiae) EG1, FKSG20, magicin, RGD1305875 MKL1 215292_s_at AI852829, megakaryoblastic 57591 223701 315151 AMKL, leukemia (translocation) 1 AW743281, AW821984, BSAC, MAL, MRTF-A MLANA 206426_at, A930034P04Rik, melan-A 2315 77836 293890 206427_s_at MART-1, MELAN-A, MGC130556 MLLT6 225628_s_at AF17, myeloid/lymphoid or 4302 246198 303504 AI315037, mixed-lineage leukemia FLJ23480 (trithorax homolog, Drosophila); translocated to, 6 MLPH 218211_s_at 2210418F23Rik, melanophilin 79083 171531 316620 5031433I09Rik, AW228792, D1Wsu84e, l(1)- 3Rk, 11Rk3, ln, MGC2771, MGC59733, SLAC2-A MYEF2 222771_s_at, 9430071B01, myelin expression factor 2 50804 17876 362207 232676_x_at FLJ11213, HsT18564, KIAA1341, MEF-2, MGC109392, MGC87325, mKIAA1341, MST156, MSTP156 MYL6B 204173_at 5730437E04Rik, myosin, light chain 6B, 140465 216459 317454 Atrial Myosin alkali, smooth muscle and Light Chain 1, non-muscle BC037527, MGC41229, MLC1SA, RGD1560334 MYO5A 227761_at 9630007J19Rik, myosin VA (heavy chain 4644 17918 25017 AI413174, 12, myoxin) AI661011, Br Myosin5a, d- 120J, Dbv, Dop, flail, flr, GS1, hcBM-V, MVa, MYH12, MYO5, myosin V, MYOSIN VA, MYOSIN VA EXON CONTAINING, MYOVA, MYOXIN, MYR12, Sev-1 NBL1 37005_at D1S1733E, neuroblastoma, 4681 17965 50594 D4H1S1733E, suppression of DAN, Dana, tumorigenicity 1 DAND1, MGC123430, MGC8972, NB, NO3 NFIB 230791_at 6720429L07Rik, nuclear factor I/B 4781 18028 29227 CTF/NF1B, E030026I10Rik, NF1-B, NFI- RED, NFIB2, NFIB3, Nuclear factor 1/B OSTM1 218196_at 1200002H13Rik, osteopetrosis associated 28962 14628 445370 AW123348, transmembrane protein 1 GIPN, GL, HSPC019 PDK3 221957_at 2610001M10Rik, pyruvate dehydrogenase 5165 236900 296849 AI035637, kinase, isozyme 3 MGC6383 PKD1 241090_at FLJ00285, polycystic kidney disease 5310 18763 24650 mFLJ00285, 1 (autosomal dominant) MGC118471, PBP, PC-1, POLYCYSTIN1 PLEKHA5 220952_s_at 2810431N21Rik, pleckstrin homology 54477 109135 246237 AI428202, domain containing, family AK129423, A member 5 Ayu21-9, FLJ10667, FLJ31492, Gt(pU21)9Imeg, Image: 3710928, KIAA1686, MGC38455, PEPP2, TRS1 PLP1 210198_s_at DM20, jimpy, jp, proteolipid protein 1 5354 18823 24943 MMPL, Msd, (Pelizaeus-Merzbacher PLP, PLP/DM20, disease, spastic paraplegia PMD, 2, uncomplicated) PROTEOLIPID, RSH, SPG2 PLXNC1 213241_at 2510048K12Rik, plexin C1 10154 54712 362873 AW742158, CD232, Plexin C1, VESPR PPP3CA 202425_x_at 2900074D19Rik, protein phosphatase 3 5530 19055 24674 AI841391, (formerly 2B), catalytic AW413465, subunit, alpha isoform Calcineurin, (calcineurin A alpha) Calcineurin A Alpha, CALN, CALNA, CALNA1, CCN1, CN, CnA, CnA- alpha, CNA1, MGC106804, Pp2b Subunit A, PPP2B PRKCSH 200707_at 80K-H, AGE- protein kinase C substrate 5589 19089 300445 R2, G19P1, 80K-H PCLD, PLD, PLD1 PRKD3 222565_s_at 4930557O20Rik, protein kinase D3 23683 75292 313834 5730497N19Rik, EPK2, MGC47171, nPKC-NU, PKC- NU, PKD3, PRKCN PRMT1 206445_s_at 6720434D09Rik, protein arginine 3276 15469 60421 ANM1, methyltransferase 1 AW214366, HCP1, heterogeneous ribonucleooproteins methyltransferase- like 2, Hnmt112, Hramt, HRMT1L2, IR1B4, Mrmt1 PSCD3 225147_at AI648983, pleckstrin homology, 9265 19159 116693 ARNO3, Sec7 and coiled-coil CYTOHESIN-3, domains 3 GRP1, KIAA4241, MGC124579, mKIAA4241, Sec7, Sec7C PTPRF 200635_s_at, AA591035, protein tyrosine 5792 19268 360406 200637_s_at FLJ43335, phosphatase, receptor FLJ45062, type, F FLJ45567, LAR, Lar ptp2b, LARFN5C, LARS PTPRM 1555579_s_at HR-PTPU, protein tyrosine 5797 19274 29616 KIAA4044, phosphatase, receptor MGC90724, type, M mKIAA4044, PTP-MU, PTPRL1, R-PTP- MU, RPTPM, RPTPU PVRL1 225211_at AI835281, poliovirus receptor- 5818 58235 192183 AW549174, related 1 (herpesvirus CD111, entry mediator C; nectin) CLPED1, ED4, HIgR, HVEC, MGC142031, MGC16207, NECTIN-1, Nectin1 alpha, Nectin1 delta, OFC7, PRR, PRR1, PVRR, PVRR1, SK-12 RAB40C 227269_s_at RAB40, RAR3, RAB40C, member RAS 57799 224624 359728 RARL, RASL8C oncogene family RASSF3 230466_s_at AW212023, Ras association 283349 192678 362886 AW322379, (RalGDS/AF-6) domain MGC119194, family 3 MGC119195, MGC119197, RASSF5 RHOQ 212120_at ARHQ, ras homolog gene family, 23433 104215 85428 RASL7A, Rhot, member Q TC10, TC10 BETA, TC10A SAT1 203455_s_at, AA617398, Ab2- spermidine/spermine N1- 6303 20229 302642 210592_s_at, 402, DC21, acetyltransferase 1 213988_s_at, KFSD, 230333_at MGC72945, SAT, Spermidine/spermine N1-acetyl transferase, SSAT, SSAT-1 SDCBP 200958_s_at MDA-9, ST1, syndecan binding protein 6386 53378 83841 SYCL, (syntenin) SYNTENIN, Syntenin-1, TACIP18 SEC61A1 217716_s_at, AA408394, Sec61 alpha 1 subunit (S. cerevisiae) 29927 53421 80843 222385_x_at AA410007, HSEC61, rSEC61alpha p, SEC61, Sec61 alpha, SEC61 ALPHA1, SEC61A SEMA3C 236947_at 1110036B02Rik, sema domain, 10512 20348 296787 SEMAE, immunoglobulin domain SEMAPHORINE, (Ig), short basic domain, SemE secreted, (semaphorin) 3C SERGEF 220482_s_at, DELGEF, Gef, secretion regulating 26297 27414 365243 232983_s_at Gnef, Gnefr, guanine nucleotide MGC141208, exchange factor MGC141209, RGD1563497 SILV 209848_s_at D10H12S53E, silver homolog (mouse) 6490 20431 362818 D12S53E, D12S53Eh, GP100, gp87, ME20, PMEL17, SI, SIL SLC2A4RG 227362_at GEF, HDBP1, SLC2A4 regulator 56731 Si-1-2, Si-1-2-19 SLC7A1 212295_s_at 4831426K01Rik, solute carrier family 7 6541 11987 25648 AI447493, (cationic amino acid ATRC1, CAT-1, transporter, y+ system), EcoR, ER, ERR, member 1 HCAT1, mCAT- 1, Rec-1, REC1L, REV-1 SRGAP2 1568957_x_at 9930124L22Rik, SLIT-ROBO Rho 23380 14270 360840 AI448945, FBP2, GTPase activating protein 2 FNBP2, KIAA0456, RGD1566016, srGAP3 SSBP3 217991_x_at, 2610021L12Rik, single stranded DNA 23648 72475 84354 223635_s_at 2610200M23Rik, binding protein 3 5730488C10Rik, AI854733, AW551939, CSDP, FLJ10355, LAST, MGC124589, SSDP, SSDP1, Ssdp3 STAM 203544_s_at DKFZp686J2352, signal transducing 8027 20844 498798 (includes RGD1564499, adaptor molecule (SH3 EG: 8027) Stam, STAM1 domain and ITAM motif) 1 SYNGR2 201079_at CELLUGYRIN, synaptogyrin 2 9144 20973 89815 Clast2, MGC102914 TCF7L2 212759_s_at mTcf-4B, mTcf- transcription factor 7-like 6934 21416 (includes 4E, TCF-4, 2 (T-cell specific, HMG- EG: 6934) TCF4B, TCF4E, box) Tcf7l2 TIMM17A 215171_s_at 17 kDa, translocase of inner 10440 21854 54311 Mitochondrial mitochondrial membrane import inner 17 homolog A (yeast) membrane translocase, Mitochondrial protein import protein 2, mTim17a, TIM17, TIM17A, Timm17 TP53 201746_at bbl, bfy, bhy, tumor protein p53 (Li- 7157 22059 24842 Delta N p53, Fraumeni syndrome) LFS1, MGC112612, P53, TRP53 TP53INP1 235602_at 2700057G22Rik, tumor protein p53 94241 60599 297822 DKFZP434M1317, inducible nuclear protein 1 FLJ22139, p53DINP1, SIP, SIP18, SIP27, Stinp, Teap, Thymus Expressed Acidic Protein, TP53DINP1, TP53DINP1alpha, TP53INP1A, TP53INP1B, Trp53inp1 TRIB2 202478_at AW319517, tribbles homolog 2 28951 217410 313974 C5fw, GS3955, (Drosophila) RGD1564451, TRB-2 TRPM1 237070_at 4732499L03Rik, transient receptor 4308 17364 (includes AI606771, potential cation channel, EG: 4308) LTRPC1, subfamily M, member 1 melastatin, MLSN, MLSN1, Trpm1 TSPAN6 209108_at 6720473L21Rik, tetraspanin 6 7105 56496 302313 AI316786, MGC117923, T245, Tm4sf, TM4SF6 TSTA3 36936_at AI256181, FX, tissue specific 7264 22122 300036 FX protein, transplantation antigen MGC113801, P35B P35B, Tstap35b TTC3 208073_x_at, 2610202A04Rik, tetratricopeptide repeat 7267 22129 360702 210645_s_at AA409221, domain 3 D16Ium21, D16Ium21e, DCRR1, DKFZp686M0150, KIAA4119, mKIAA4119, Mtprd, RNF105, TPRD, TPRDIII TUBB4 212664_at AI325297, Beta tubulin, beta 4 10382 22153 29213 tubulin, BETA TUBULIN 4 ALPHA, Beta tubulin class iv, beta-5, Beta4 Tubulin, M(beta)4, Tubb, TUBB5, TUBULIN BETA (5-BETA), TUBULIN BETA5 TYR 206630_at albino, Dopa tyrosinase 7299 22173 308800 oxidase, (oculocutaneous albinism Melanogenesis IA) Related Tyrosinase, OCA1A, OCAIA, skc35, Tyr&lt; c- em&gt;, TYROSINASE TYRP1 205694_at b-PROTEIN, tyrosinase-related protein 1 7306 22178 298182 brown, CAS2, CATB, GP75, isa, MELANOMA ANTIGEN GP75, TRP, TRP-1, TYRP VDR 204255_s_at NR1I1, VD3R, vitamin D (1,25- 7421 22337 24873 VITAMIN D dihydroxyvitamin D3) RECEPTOR receptor VGLL4 214004_s_at BC048841, vestigial like 4 9686 232334 297523 KIAA0121, (Drosophila) MGC109514, MGC54805, VGL-4 YIPF5 224949_at 2610311I19Rik, Yip1 domain family, 81555 67180 361315 AA408236, Ac2- member 5 256, DKFZp313L2216, FinGER5, SB140, SMAP-5, YIP1A ZFHX1B 1557797_a_at, 9130203F04Rik, zinc finger homeobox 1b 9839 24136 311071 203603_s_at D130016B08Rik, KIAA0569, mKIAA0569, SIP-1, SMADIP1, ZEB2, Zfx1b, Zfxh1b 1558019_at —: Homo sapiens, clone IMAGE: 4732650, mRNA 233551_at LOC642776: hypothetical protein LOC642776 208646_at RPS14: ribosomal protein S14 /// similar to ribosomal protein S14 208929_x_at RPL13: ribosomal protein L13 214351_x_at RPL13: ribosomal protein L13 /// similar to ribosomal protein L13 200817_x_at RPS10: ribosomal protein S10 213296_at —: Transcribed locus 213692_s_at —: — 227957_at —: — 232462_s_at FLJ23569:BC040926 227722_at RPS23: ribosomal protein S23 217466_x_at RPS2: ribosomal protein S2 /// similar to ribosomal protein S2 235534_at —: Homo sapiens, clone IMAGE: 5723825, mRNA 230741_at —: Full length insert cDNA clone YX74D05 229067_at LOC653464: Similar to SLIT- ROBO Rho GTPase- activating protein 2 (srGAP2) (Formin0binding protein 2)

TABLE 2 name matched term ANKRD44 228471_at ARHGEF19 226857_at ATPBD4 238662_at BARX2 210419_at BDNF 206382_s_at BLOC1S1 202592_at C16ORF48 223407_at C6ORF218 244829_at C8ORF13 233641_s_at CCHCR1 37425_g_at CIRBP 230142_s_at CLSTN2 219414_at COL7A1 217312_s_at DACH1 205472_s_at, 228915_at DCT 205337_at, 205338_s_at DOCK10 219279_at DRAP1 1556181_at EDNRB 204271_s_at, 206701_x_at EFNA4 205107_s_at EHD2 45297_at ETS1 224833_at FAM33A 225684_at FGFR1 210973_s_at, 211535_s_at FOXO1A 202723_s_at GGA3 209411_s_at GPR161 214104_at HIST2H2AA3 214290_s_at ID1 208937_s_at KDELR1 200922_at KIAA0738 210529_s_at KIT 205051_s_at LGR4 230674_at LHX2 (includes EG: 9355) 211219_s_at LMO4 209204_at LOC254100 1557131_at LRIG1 238339_x_at MED28 222635_s_at MKL1 215292_s_at MLANA 206426_at, 206427_s_at MLPH 218211_s_at MYEF2 222771_s_at, 232676_x_at MYO5A 227761_at NBL1 37005_at OSTM1 218196_at PDK3 221957_at PKD1 241090_at PLEKHA5 220952_s_at PLP1 210198_s_at PLXNC1 213241_at PRKCSH 200707_at PRKD3 222565_s_at PRMT1 206445_s_at PSCD3 225147_at PTPRF 200637_s_at PTPRM 1555579_s_at RAB40C 227269_s_at RASSF3 230466_s_at RHOQ 212120_at RPL13 214351_x_at RPS23 227722_at SAT1 203455_s_at, 213988_s_at, 230333_at SDCBP 200958_s_at SEC61A1 222385_x_at SEMA3C 236947_at SERGEF 232983_s_at SILV 209848_s_at SLC2A4RG 227362_at SLC7A1 212295_s_at SSBP3 217991_x_at, 223635_s_at STAM (includes EG: 8027) 203544_s_at SYNGR2 201079_at TCF7L2 (includes EG: 6934) 212759_s_at TIMM17A 215171_s_at TRIB2 202478_at TRPM1 (includes EG: 4308) 237070_at TSPAN6 209108_at TTC3 208073_x_at, 210645_s_at TUBB4 212664_at TYR 206630_at VDR 204255_s_at YIPF5 224949_at ZFHX1B 1557797_a_at, 203603_s_at 229067_at 213692_s_at 227957_at 213296_at 235534_at 233551_at 1558019_at

TABLE 3 matched term description 208073_x_at TTC3: tetratricopeptide repeat domain 3 210645_s_at TTC3: tetratricopeptide repeat domain 3 206630_at TYR: tyrosinase (oculocutaneous albinism IA) 203544_s_at STAM: signal transducing adaptor molecule (SH3 domain and ITAM motif) 1 230741_at —: Full length insert cDNA clone YX74D05

TABLE 4 matched term description 205694_at TYRP1: tyrosinase-related protein 1 206427_s_at MLANA: melan-A 206140_at LHX2: LIM homeobox 2 206630_at TYR: tyrosinase (oculocutaneous albinism IA) 203921_at CHST2: carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2 205337_at DCT: dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2) 228245_s_at OVOS2: ovostatin 2 /// similar to cDNA sequence BC048546 205338_s_at DCT: dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2) 1557797_a_at ZFHX1B: Zinc finger homeobox 1b 204271_s_at EDNRB: endothelin receptor type B 237070_at TRPM1: transient receptor potential cation channel, subfamily M, member 1 200716_x_at RPL13A: ribosomal protein L13a 1555579_s_at PTPRM: protein tyrosine phosphatase, receptor type, M 205051_s_at KIT: v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog 200665_s_at SPARC: secreted protein, acidic, cysteine-rich (osteonectin) /// secreted protein, acidic, cysteine-rich (osteonectin) 205174_s_at QPCT: glutaminyl-peptide cyclotransferase (glutaminyl cyclase) 200725_x_at RPL10: ribosomal protein L10 232602_at WFDC3: WAP four-disulfide core domain 3 202478_at TRIB2: tribbles homolog 2 (Drosophila) 209230_s_at P8: p8 protein (candidate of metastasis 1) 232676_x_at MYEF2: myelin expression factor 2 222565_s_at PRKD3: protein kinase D3 212295_s_at SLC7A1: solute carrier family 7 (cationic amino acid transporter, y+ system), member 1 212594_at PDCD4: programmed cell death 4 (neoplastic transformation inhibitor) 218211_s_at MLPH: melanophilin 206426_at MLANA: melan-A 207065_at K6HF: cytokeratin type II 202500_at DNAJB2: DnaJ (Hsp40) homolog, subfamily B, member 2 203706_s_at FZD7: frizzled homolog 7 (Drosophila) 209969_s_at STAT1: signal transducer and activator of transcription 1, 91 kDa

TABLE 5 matched term description 205694_at tyrosinase-related protein 1 206140_at LIM homeobox 2 206427_s_at melan-A 203455_s_at spermidine/spermine N1-acetyltransferase 206453_s_at NDRG family member 2 203921_at carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2 200958_s_at syndecan binding protein (syntenin) 209283_at crystallin, alpha B 204271_s_at endothelin receptor type B 208073_x_at tetratricopeptide repeat domain 3 232602_at WAP four-disulfide core domain 3 202435_s_at cytochrome P450, family 1, subfamily B, polypeptide 1 209230_s_at p8 protein (candidate of metastasis 1) 208966_x_at interferon, gamma-inducible protein 16 205337_at dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2) 202088_at solute carrier family 39 (zinc transporter), member 6 211538_s_at heat shock 70 kDa protein 2 201556_s_at vesicle-associated membrane protein 2 (synaptobrevin 2) 241455_at Similar to AI661453 protein 237070_at transient receptor potential cation channel, subfamily M, member 1

TABLE 6 matched term description 1555505_a_at tyrosinase (oculocutaneous albinism IA) 204271_s_at endothelin receptor type B 208073_x_at tetratricopeptide repeat domain 3 200958_s_at syndecan binding protein (syntenin) 205051_s_at v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog 201245_s_at OTU domain, ubiquitin aldehyde binding 1 201603_at protein phosphatase 1, regulatory (inhibitor) subunit 12A 201605_x_at calponin 2 201908_at dishevelled, dsh homolog 3 (Drosophila) 202478_at tribbles homolog 2 (Drosophila) 1557292_a_at mucolipin 3 200601_at actinin, alpha 4 200819_s_at ribosomal protein S15 209953_s_at CDC37 cell division cycle 37 homolog (S. cerevisiae) 213146_at jumonji domain containing 3 222670_s_at v-maf musculoaponeurotic fibrosarcoma oncogene homolog B (avian) 224991_at c-Maf-inducing protein 226988_s_at myosin, heavy polypeptide 14 244829_at Hypothetical protein MGC40222

Although the invention has been described with reference to the above examples, it will be understood that modifications and variations are encompassed within the spirit and scope of the invention. Accordingly, the invention is limited only by the following claims. 

1. A method for characterizing a skin lesion in a subject comprising analyzing a nucleic acid molecule from one or more genes listed in any of Tables 1-6, or any combination thereof, in a sample of the skin lesion, thereby characterizing a skin lesion of the subject.
 2. The method of claim 1, wherein the nucleic acid molecule is RNA.
 3. The method of claim 1, wherein analyzing the nucleic acid molecule comprises detecting one or more mutations in the nucleic acid sequence of the nucleic acid molecule.
 4. The method of claim 3, wherein the one or more mutations are selected from the group consisting of a substitution, a deletion, and an insertion.
 5. The method of claim 1, further comprising amplifying the nucleic acid molecule obtained from the sample prior to analyzing.
 6. The method of claim 1, wherein the sample is obtained by applying an adhesive tape to a target area of skin in a manner sufficient to isolate the sample adhering to the adhesive tape.
 7. The method of claim 1, further comprising using the characterizing to determine a treatment regimen.
 8. The method of claim 2, wherein the isolated nucleic acid molecule or an amplification product thereof, is applied to a microarray.
 9. The method of claim 8, wherein an expression profile is detected using a microarray.
 10. The method of claim 1, wherein the sample is obtained from a biopsy taken at the site of the skin lesion or surrounding margin.
 11. The method of claim 6, wherein the tape comprises a rubber adhesive on a polyurethane film.
 12. The method of claim 6, wherein about one to ten adhesive tapes or one to ten applications of a tape are applied and removed from the skin.
 13. The method of claim 6, wherein about one to eight adhesive tapes or one to eight applications of a tape are applied and removed from the skin.
 14. The method of claim 6, wherein about one to five adhesive tapes or one to five applications of a tape are applied and removed from the skin.
 15. The method of claim 6, wherein the method further comprises taking a biopsy of the target area of the skin.
 16. The method of claim 2, wherein the analyzing is performed in situ.
 17. The method of claim 1, wherein the nucleic acid molecule is from one or more genes listed in Table
 6. 18. A method of distinguishing melanoma from dysplastic nevi or normal pigmented skin in a subject comprising analyzing a nucleic acid molecule from one or more genes listed in any of Tables 1-6, or any combination thereof, in a sample from the subject, thereby distinguishing melanoma from dysplastic nevi or normal pigmented skin in a subject.
 19. The method of claim 18, wherein the nucleic acid molecule is RNA.
 20. The method of claim 18, wherein analyzing the nucleic acid molecule comprises detecting one or more mutations in the nucleic acid sequence of the nucleic acid molecule.
 21. The method of claim 20, wherein the one or more mutations are selected from the group consisting of a substitution, a deletion, and an insertion.
 22. The method of claim 18, further comprising amplifying the nucleic acid molecule obtained from the sample prior to analyzing.
 23. The method of claim 18, wherein the sample is obtained by applying an adhesive tape to a target area of skin in a manner sufficient to isolate the sample adhering to the adhesive tape, wherein the sample comprises nucleic acid molecules.
 24. The method of claim 19, wherein the isolated nucleic acid molecule or an amplification product thereof, is applied to a microarray.
 25. The method of claim 22, wherein an expression profile is detected using a microarray.
 26. The method of claim 18, wherein the sample is obtained from a biopsy taken from a target area of skin from the subject.
 27. The method of claim 23, wherein the tape comprises a rubber adhesive on a polyurethane film.
 28. The method of claim 23, wherein about one to ten adhesive tapes or one to ten applications of a tape are applied and removed from the skin.
 29. The method of claim 23, wherein about one to eight adhesive tapes or one to eight applications of a tape are applied and removed from the skin.
 30. The method of claim 23, wherein about one to five adhesive tapes or one to five applications of a tape are applied and removed from the skin.
 31. The method of claim 23, wherein the method further comprises taking a biopsy of the target area of the skin.
 32. The method of claim 19, wherein the analyzing is performed in situ.
 33. A method for diagnosing melanoma in a subject comprising detecting an altered level of a target protein in a sample from the subject, as compared to the level of the target protein in a corresponding sample from a subject that does not have melanoma, wherein the protein is an expression product of a gene listed in any of Tables 1-6, or any combination thereof, thereby diagnosing melanoma in the subject.
 34. The method of claim 33, wherein the sample is obtained by applying an adhesive tape to a target area of skin in a manner sufficient to isolate the sample adhering to the adhesive tape, wherein the sample comprises cells, and further comprising lysing the cells to extract the target protein.
 35. The method of claim 34, wherein the tape comprises a rubber adhesive on a polyurethane film.
 36. The method of claim 34, wherein between one and ten adhesive tapes are applied to the skin and removed from the skin.
 37. The method of claim 34, wherein about one to eight adhesive tapes are applied and removed from the skin.
 38. The method of claim 34, wherein about one to five adhesive tapes are applied and removed from the skin.
 39. The method of claim 34, wherein the method further comprises taking a biopsy of the target area of the skin.
 40. The method of claim 39, wherein protein is extracted from the biopsy sample, and the level of protein in the biopsy and the level of protein in the tape sample are analyzed.
 41. The method of claim 33, wherein the sample is obtained by from a biopsy of a target area of skin.
 42. The method of claim 33, further comprising obtaining a sample from uninvolved tissue of the subject.
 43. The method of claim 42, wherein the sample from uninvolved tissue is obtained by taking a biopsy of the uninvolved skin.
 44. The method of claim 42, wherein the sample from uninvolved tissue is obtained by: a) applying an adhesive tape to skin of the subject in a manner sufficient to isolate a skin sample adhering to the adhesive tape, wherein the skin sample comprises cells from the stratum corneum and wherein the skin is unaffected by a disease to be tested; b) lysing the cells to extract a protein; and c) quantitating the extracted protein.
 45. The method of claim 42, wherein the uninvolved skin is from the mastoid process or the upper back.
 46. The method of claim 33, wherein the protein is an expression product of a gene listed in Table
 6. 47. A method for diagnosing melanoma in a subject, comprising: a) providing a gene expression profile of a target area suspected of being melanoma on the skin of the subject, wherein the target area of the skin simultaneously expresses a plurality of genes at the protein level that are markers for melanoma; and b) comparing the subject's gene expression profile to a reference gene expression profile obtained from a corresponding normal skin sample, wherein the reference gene expression profile comprises an expression value of a target gene selected from the group consisting of human mRNA for tyrosinase-related protein 1, LIM homeobox 2, melan-A, spermidine/spermine N1-acetyltransferase, NDRG family member 2, carbohydrate (N-acetylglucosamine-6-O) sulfotransferase 2, syndecan binding protein (syntenin), crystallin, alpha B, endothelin receptor type B, tetratricopeptide repeat domain 3, WAP four-disulfide core domain 3, cytochrome P450 (family 1, subfamily B, polypeptide 1), p8 protein (candidate of metastasis 1), interferon gamma-inducible protein 16, dopachrome tautomerase (dopachrome delta-isomerase, tyrosine-related protein 2), solute carrier family 39 (zinc transporter), member 6, heat shock 70 kDa protein 2, vesicle-associated membrane protein 2 (synaptobrevin 2), Similar to AI661453 protein, and transient receptor potential cation channel (subfamily M, member 1), tyrosinase (oculocutaneous albinism IA), endothelin receptor type B, tetratricopeptide repeat domain 3, syndecan binding protein (syntenin), v-kit Hardy-Zuckerman 4 feline sarcoma viral oncogene homolog, OTU domain, ubiquitin aldehyde binding 1, protein phosphatase 1 regulatory (inhibitor) subunit 12A, calponin 2, dishevelled dsh homolog 3 (Drosophila), tribbles homolog 2 (Drosophila), mucolipin 3, actinin alpha 4, ribosomal protein S15, CDC37 cell division cycle 37 homolog (S. cerevisiae), jumonji domain containing 3, v-maf musculoaponeurotic fibrosarcoma oncogene homolog B (avian), c-Maf-inducing protein, myosin heavy polypeptide 14, Hypothetical protein MGC40222, or any combination thereof.
 48. The method of claim 47, wherein the reference gene expression profile further comprises an expression value of any target gene listed in Tables 1-6.
 49. The method of claim 47 or 48, wherein the reference gene expression profile is contained within a database.
 50. The method of claim 47, wherein said comparing is carried out using a computer algorithm.
 51. A kit for characterizing a skin lesion in a subject comprising a skin sample collection device and one or more probes or primers that selectively bind to one or more nucleic acid molecules in any of Tables 1-6, or to a nucleic acid or protein expression product of a nucleic acid molecule in any of Tables 1-6.
 52. The kit of claim 51, wherein the kit provides a probe which binds to a portion of a nucleic acid molecule in any of Tables 1-6.
 53. The kit of claim 51, wherein the kit provides one or more primer pairs comprising a forward primer that selectively binds upstream of a gene on one strand and a reverse primer that selectively binds upstream of a gene on a complementary strand, wherein the gene is listed in any of Tables 1-6.
 54. The kit of claim 51, wherein the skin sample collection device is a biopsy needle.
 55. The kit of claim 51, wherein the skin sample collection device is an adhesive tape.
 56. The kit of claim 55, wherein the adhesive tape comprises a rubber adhesive on a polyurethane film.
 57. The kit of claim 51, further comprising a microarray containing at least a fragment of a gene or a nucleic acid or protein product of a gene identified in any of Tables 1-6 or any combination thereof.
 58. A kit for characterizing a skin lesion in a subject comprising an applicator and one or more probes or primers that selectively bind to one or more of nucleic acid molecules in any of Tables 1-6, or to a nucleic acid or protein expression product of a nucleic acid molecule in any of Tables 1-6.
 59. The kit of claim 58, wherein the probes are detectably labeled.
 60. The method of any one of claims 1, 18, 33, or 47, wherein the subject is human.
 61. The method of any one of claims 1, 18, 33, or 47, wherein the sample is an epidermal sample. 